.
The cytosol ( gray), endoplasmic reticulum, Golgi apparatus, nucleus, mitochondrion, endosome, lysosome, and peroxisome are distinct compartments isolated from the rest of the cell by at least one selectively permeable membrane.
 |
Unlike a bacterium, which generally consists of a single intracellular compartment surrounded by a plasma membrane, a eucaryotic cell is elaborately subdivided into functionally distinct, membrane-bounded compartments. Each compartment, or organelle, contains its own characteristic set of enzymes and other specialized molecules, and complex distribution systems transport specific products from one compartment to another. To understand the eucaryotic cell, it is essential to know what occurs in each of these compartments, how molecules move between them, and how the compartments themselves are created and maintained.
Proteins play a central part in the compartmentalization of a eucaryotic cell. They catalyze the reactions that occur in each organelle and selectively transport small molecules into and out of its interior, or lumen. Proteins also serve as organelle-specific surface markers that direct new deliveries of proteins and lipids to the appropriate organelle. A mammalian cell contains about 10 billion (10 10) protein molecules of perhaps 10,000 kinds, and the synthesis of almost all of them begins in the cytosol. Each newly synthesized protein is then delivered specifically to the cell compartment that requires it. We shall make the intracellular transport of proteins the central theme of this chapter as well as of the next. By tracing the protein traffic from one compartment to another, one can begin to make sense of the otherwise bewildering maze of intracellular membranes.
In this introductory section we give a brief overview of the compartments of the cell and of the relationships between them. In doing so, we organize the organelles conceptually into a small number of discrete families, discussing how proteins are directed to specific organelles and how they cross organelle membranes.
Many vital biochemical processes take place in or on membrane surfaces. Lipid metabolism, for example, is catalyzed mostly by membrane-bound enzymes, and oxidative phosphorylation and photosynthesis both require a membrane in order to couple the transport of H + to the synthesis of ATP. Intracellular membrane systems, however, do more for the cell than just provide increased membrane area: they create enclosed compartments that are separate from the cytosol, thus providing the cell with functionally specialized aqueous spaces. Because the lipid bilayer of organelle membranes is impermeable to most hydrophilic molecules, the membrane of each organelle must contain transport proteins that are responsible for the import and export of specific metabolites. Each organelle membrane must also have a mechanism for importing, and incorporating into the organelle, the specific proteins that make the organelle unique.
The cytosol ( gray), endoplasmic reticulum, Golgi apparatus, nucleus, mitochondrion, endosome, lysosome, and peroxisome are distinct compartments isolated from the rest of the cell by at least one selectively permeable membrane.
. The nucleus contains the main genome and is the
principal site of DNA and RNA synthesis. The surrounding cytoplasm consists of the cytosol and the cytoplasmic
organelles suspended in it. The cytosol
constitutes a little more than half the total volume of the cell and is the
site of protein
synthesis and of most of the cell's intermediary metabolism - that is, the
many
reactions by which some small molecules are degraded and others are
synthesized to provide the building blocks of macromolecules (discussed in Chapter 2).
About half the total area of membrane in a cell encloses the labyrinthine spaces of the endoplasmic reticulum (ER). The ER has many ribosomes bound to its cytosolic surface; these are engaged in the synthesis of integral membrane proteins and soluble proteins, most of which are destined for secretion or for other organelles. We shall see that this reflects an important difference between how proteins are directed to the ER and how they are directed to other cytoplasmic organelles: whereas proteins are translocated into other organelles only after their synthesis is complete, they are translocated into the ER during their synthesis, and hence the ribosomes on which they are made are tethered to the ER membrane. The ER also produces the lipid for the rest of the cell and functions as a store for Ca 2+ ions. The Golgi apparatus consists of organized stacks of disclike compartments called Golgi cisternae; it receives lipids and proteins from the ER and dispatches them to a variety of destinations, usually covalently modifying them en route .
Mitochondria and (in plants) chloroplasts generate most of the ATP used to drive cellular reactions that require an input of free energy. Lysosomes contain digestive enzymes that degrade defunct intracellular organelles, as well as macromolecules and particles taken in from outside the cell by endocytosis. On their way to lysosomes, endocytosed material must first pass through a series of compartments called endosomes. Peroxisomes (also known as microbodies) are small vesicular compartments that contain enzymes utilized in a variety of oxidative reactions. In general, each membrane-bounded organelle carries out the same set of basic functions in all cell types but varies in abundance and can have additional properties that differ from cell type to cell type according to the specialized functions of differentiated cells.
| Intracellular Compartment | Percent of Total Cell Volume | Approximate Number per Cell* |
|---|---|---|
| Cytosol | 54 | 1 |
| Mitochondria | 22 | 1700 |
| Rough ER cisternae | 9 | 1 |
| Smooth ER cisternae plus Golgi cisternae | 6 | |
| Nucleus | 6 | 1 |
| Peroxisomes | 1 | 400 |
| Lysosomes | 1 | 300 |
| Endosomes | 1 | 200 |
All the cisternae of the rough and smooth endoplasmic reticulum are thought to be joined to form a single large compartment. The Golgi apparatus, in contrast, is organized into a number of discrete sets of stacked cisternae in each cell, and the extent of interconnection between these sets has not been clearly established.
| Percent of Total Cell Membrane | ||
|---|---|---|
| Membrane Type | Liver Hepatocyte* | Pancreatic Exocrine Cell* |
| Plasma membrane | 2 | 5 |
| Rough ER membrane | 35 | 60 |
| Smooth ER membrane | 16 | <1 |
| Golgi apparatus membrane | 7 | 10 |
| Mitochondria | ||
 Outer membrane | 7 | 4 |
| Inner membrane | 32 | 17 |
| Nucleus | ||
| Inner membrane | 0.2 | 3 |
| Secretory vesicle membrane | not determined | 3 |
| Lysosome membrane | 0.4 | not determined |
| Peroxisome membrane | 0.4 | not determined |
| Endosome membrane | 0.4 | not determined |
These two cells are of very different sizes, since the average hepatocyte has a volume of about 5000 µ m 3compared with about 1000 µ m 3for the pancreatic exocrine cell. Total cell membrane areas are estimated at about 110,000 µ m 2 and 13,000 µ m 2, respectively.
Examples of most of the major intracellular compartments are indicated. (Courtesy of Daniel S. Friend.)
).
Membrane-bounded organelles are not randomly distributed in the cytosol; instead they often have characteristic positions. In most cells, for example, the Golgi apparatus is located close to the nucleus, whereas the network of ER tubules extends from the nucleus throughout the entire cytosol. These characteristic distributions seem to depend on interactions of the organelles with the cytoskeleton: the localization of both the ER and the Golgi apparatus, for example, is dependent on an intact microtubule array; if the microtubules are experimentally depolymerized with a drug, the Golgi apparatus fragments and disperses throughout the cell and the ER network collapses toward the cell center, or centrosome, from which the microtubule array emanates (discussed in Chapter 16).
To understand the relationships between the compartments of the cell, it is helpful to consider how they might have evolved. The precursors of the first eucaryotic cells are thought to have been simple organisms that resembled bacteria, which generally have a plasma membrane but no internal membranes. The plasma membrane in such cells therefore provides all membrane-dependent functions, including the pumping of ions, ATP synthesis, protein secretion, and lipid synthesis. Typical present-day eucaryotic cells are 10 to 30 times larger in linear dimension and 1000 to 10,000 times greater in volume than a typical bacterium such as E. coli. The profusion of internal membranes can be seen in part as an adaptation to this increase in size: the eucaryotic cell has a much smaller ratio of surface to volume, and its area of plasma membrane is presumably too small to sustain the many vital functions for which membranes are required.
(A) Membrane patches on the cell surface consisting of clusters of specialized membrane proteins. (B) Invaginated patches of plasma membrane that increase the amount of membrane available for a specialized function such as photosynthesis. (C) Internalization of the specialized invaginated membrane to form vesicles, whose interior surface is topologically equivalent to the exterior surface of the cell. Membrane-bounded vesicles of this type are present in some types of photosynthetic bacteria; their topological relationship to the cell surface is similar to that of the ER, Golgi apparatus, endosomes, and lysosomes in eucaryotic cells.
). These
specialized membrane patches, such as the "purple membrane"
containing
bacterio-rhodopsin in Halobacterium (discussed in Chapter 10)
and the
chromatophores in photosynthetic bacteria (discussed in Chapter 14),
represent primitive
organelles. In some photosynthetic bacteria the patches have become
elaborated into extensive invaginations of the plasma membrane ( Figure 12-3B); in
others the invaginations seem to have pinched off completely, forming sealed
membrane-bounded vesicles specialized for photosynthesis ( Figure 12-3C).
Topologically equivalent spaces are shown in red. In principle, cycles of vesicle budding and fusion permit any lumen to communicate with any other and with the cell exterior. The blue arrows indicate the outward direction of vesicle traffic from the ER to Golgi apparatus to plasma membrane (or lysosomes), and the black dots represent protein molecules that are secreted by the cell. Some organelles, most notably mitochondria and (in plant cells) chloroplasts, however, do not take part in this vesicular communication and so are isolated from the traffic between organelles shown here.
might be expected to have an
interior that is topologically
equivalent to the exterior of the cell. We shall see that this is the case
for the ER,
Golgi apparatus, endosome, and lysosome - as well as for the many vesicular
intermediates ( transport vesicles) in the secretory and
endocytic pathways. We can
therefore think of all of these organelles as members of the same family,
and, as
we discuss in detail in the next chapter, their interiors communicate
extensively
with one another and with the outside of the cell via transport vesicles
that bud
off from one organelle and fuse with another ( Figure 12-4). Ribosomes are
found attached to the cytosolic side of the plasma membrane in bacteria,
and so
the evolutionary origin of the ER membrane from the plasma membrane may
explain why ribosomes are attached to the ER membrane in eucaryotic cells.
The origins of mitochondria, chloroplasts, ER, and the cell nucleus could explain the topological relationships of these intracellular compartments in eucaryotic cells. (A) A possible pathway for the evolution of the cell nucleus and the ER. In some bacteria the single DNA molecule is attached to an invagination of the plasma membrane, called a mesosome. Such an invagination in a very ancient procaryotic cell could have spread to form an envelope around the DNA while still allowing access of the DNA to the cell cytosol (as is required for DNA to direct protein synthesis). This envelope is presumed to have eventually pinched off completely from the plasma membrane, producing a nuclear compartment surrounded by a double membrane. As illustrated, the nuclear envelope is organized by a fibrous shell called the nuclear lamina and is penetrated by communicating channels called nuclear pore complexes. Because it is surrounded by two membranes that are in continuity where they are penetrated by these pores, the nuclear compartment is topologically equivalent to the cytosol. The lumen of the ER is continuous with the space between the inner and outer nuclear membranes and topologically equivalent to the extracellular space. (B) Mitochondria (and chloroplasts) are thought to have originated when a bacterium was engulfed by a larger pre-eucaryotic cell. They retain their autonomy. This may explain why the lumens of these organelles remain isolated from the vesicular traffic that interconnects the lumens of many other intracellular compartments.
. This
scheme would explain why the nuclear compartment is topologically
equivalent to
the cytosol. In fact, in higher eucaryotic cells the nuclear envelope breaks
down during mitosis, allowing the nuclear contents to disperse in the
cytosol, a
situation that never occurs for the contents of any other membrane-bounded
organelle. As the scheme in Figure 12-5A also
predicts, the space between the
two nuclear membranes is topologically equivalent to the exterior of the
cell and
is continuous with the lumen of the ER.
, the inner membrane of mitochondria and
plastids corresponds to the
original plasma membrane of the bacterium, while the lumen of these
organelles
evolved from the bacterial cytosol. As might be expected from such origins,
these
two organelles remain isolated from the extensive vesicular traffic that
connects
the interiors of most of the other membrane-bounded organelles to one another
and to the outside of the cell.
This evolutionary scheme groups the intracellular compartments in eucaryotic cells into five distinct families: (1) the nucleus and the cytosol, which communicate through the nuclear pores and are thus topologically continuous (although functionally distinct); (2) all organelles that function in the secretory and endocytic pathways - including the ER, Golgi apparatus, endosomes, lysosomes, and numerous classes of transport vesicles; (3) the mitochondria; (4) the plastids (in plants only); and (5) the peroxisomes (whose evolutionary origins are discussed later).
All proteins begin being synthesized on ribosomes in the cytosol, except for the few that are synthesized on the ribosomes of mitochondria and plastids. Their subsequent fate depends on their amino acid sequence, which can contain sorting signals that direct their delivery to locations outside the cytosol. Most proteins do not have a sorting signal and consequently remain in the cytosol as permanent residents. Many others, however, have specific sorting signals that direct their transport from the cytosol into the nucleus, the ER, mitochondria, plastids (in plants), or peroxisomes; sorting signals can also direct the transport of proteins from the ER to other destinations in the cell.
Note that the original orientation of both proteins and lipids in the donor-compartment membrane is preserved in the target-compartment membrane and that soluble molecules are transferred from lumen to lumen.
Proteins can move from one compartment to another by gated transport ( red), trans-membrane transport ( blue), or vesicular transport ( green). The signals that direct a given protein's movement through the system, and thereby determine its eventual location in the cell, are contained in its amino acid sequence. The journey begins with the synthesis of a protein on a ribosome and terminates when the final destination is reached. At each intermediate station ( boxes) a decision is made as to whether the protein is to be retained or transported further. In principle, a signal could be required either for retention in or for exit from each of the compartments shown, with the alternative fate being the default pathway (one that requires no signal). The vesicular transport of proteins from the ER through the Golgi apparatus to the cell surface, for example, appears not to require any specific sorting signals; specific sorting signals therefore are required to retain in the ER and the Golgi apparatus those specialized proteins that are resident there.
We shall use this figure repeatedly as a guide throughout this chapter and the next, highlighting the particular pathway being discussed.
). We
discuss vesicular transport in more detail in Chapter 13. The three ways in
which proteins are transported between different compartments are summarized
in Figure 12-7.
Each of the three modes of protein transfer is usually selectively guided by sorting signals in the transported protein that are recognized by complementary receptor proteins in the target organelle. If a large protein is to be imported into the nucleus, for example, it must possess a sorting signal that is recognized by receptor proteins associated with the nuclear pore complex. If a protein is to be transferred directly across a membrane, it must possess a sorting signal that is recognized by the translocator in the membrane to be crossed. Likewise, if a protein is to be incorporated into certain types of transport vesicles or to be retained in certain organelles, its sorting signal must be recognized by a complementary receptor in the appropriate membrane.
(A) The signal resides in a single discrete stretch of amino acid sequence, called a signal peptide,that is exposed in the folded protein. Signal peptides often occur at the end of the polypeptide chain (as shown), but they can also be located elsewhere. (B) A signal patch can be formed by the juxtaposition of amino acids from regions that are physically separated before the protein folds (as shown); alternatively, separate patches on the surface of the folded protein that are spaced a fixed distance apart could form the signal. In either case the transport signal depends on the three-dimensional conformation of the protein, which makes it difficult to locate the signal precisely.
). Signal peptides are used to direct
proteins from the cytosol into the
ER, mitochondria, chloroplasts, peroxisomes, and nucleus, and they are also
used
to retain soluble proteins in the ER. Signal patches identify certain
enzymes that
are to be marked with specific sugar residues that then direct them from the
Golgi apparatus into lysosomes; signal patches are also used in other
sorting steps
that have been less well characterized.
Different types of signal peptides are used to specify different destinations in the cell. Proteins destined for initial transfer to the ER usually have a signal peptide at their amino terminus, which characteristically includes a sequence composed of about 5 to 10 hydrophobic amino acids. Most of these proteins will in turn pass from the ER to the Golgi apparatus, but those with a specific sequence of four amino acids at their carboxyl terminus are retained as permanent ER residents. Proteins destined for mitochondria have signal peptides of yet another type, in which positively charged amino acids alternate with hydrophobic ones. Proteins destined for peroxisomes usually have a specific signal sequence of three amino acids at their carboxyl terminus. Many proteins destined for the nucleus carry a signal peptide formed from a cluster of positively charged amino acids, which is commonly found at internal sites of the polypeptide chain. Some typical signal peptides are listed in Table 12-3.
The importance of each of these signal peptides for protein targeting has been shown by experiments in which the peptide is transferred from one protein to another by genetic engineering techniques: placing the amino-terminal ER signal peptide at the beginning of a cytosolic protein, for example, redirects the protein to the ER. Even though their amino acid sequences can vary greatly, the signal peptides of all proteins having the same destination are functionally interchangeable: physical properties, such as hydrophobicity, often appear to be more important in the signal-recognition process than the exact amino acid sequence.
Signal patches are far more difficult to analyze than signal peptides, and so less is known about their structure. Because they result from a complex three-dimensional protein-folding pattern, they cannot be easily transferred experimentally from one protein to another.
The main ways of studying how proteins are directed from the cytosol to a specific compartment and how they are translocated across membranes are illustrated in Panel 12-1 (pp. 559).
When a cell reproduces by division, it has to duplicate its membrane-bounded organelles. In general, cells do this by enlarging the existing organelles by incorporating new molecules into them; the enlarged organelles then divide and are distributed to the two daughter cells. Thus each daughter cell inherits from its mother a complete set of specialized cell membranes. This inheritance is essential because a cell could not make such membranes de novo. If the ER were completely removed from a cell, for example, how could the cell reconstruct it? The membrane proteins that define the ER and carry out many of its functions are themselves products of the ER. A new ER could not be made without an existing ER or, at the very least, a membrane that contains the translocators required to import specific proteins into the ER (and lacks the translocators required to import the proteins that function in other organelles).
Thus it seems that the information required to construct a membrane-bounded organelle does not reside exclusively in the DNA that specifies the organelle's proteins. Epigeneticinformation in the form of at least one distinct protein that preexists in the organelle membrane is also required, and this information is passed from parent cell to progeny cell in the form of the organelle itself. Presumably, such information is essential for the propagation of the cell's compartmental organization, just as the information in DNA is essential for the propagation of its nucleotide and amino acid sequences.
Eucaryotic cells contain intracellular membranes that enclose nearly half the cell's total volume in separate intracellular compartments called organelles. The main types of membrane-bounded organelles that are present in all eucaryotic cells are the endoplasmic reticulum, Golgi apparatus, nucleus, mitochondria, lysosomes, endosomes, and peroxisomes; plant cells also contain plastids, such as chloroplasts. Each organelle contains a distinct set of proteins that mediates its unique functions.
Each newly synthesized organelle protein finds its way from the ribosome where it is made to the organelle where it functions by following a specific pathway, guided by signals in its amino acid sequence that function as signal peptides or signal patches. The signal peptides and patches are recognized by complementary receptor proteins in the target organelle. Proteins that function in the cytosol do not contain signal peptides or signal patches and therefore remain in the cytosol after they are synthesized.
The double-membrane envelope is penetrated by nuclear pores and is continuous with the endoplasmic reticulum. The ribosomes that are bound to the cytosolic surface of the ER membrane and outer nuclear membrane are not shown.
). Like the membrane
of the rough ER, the outer nuclear membrane is studded with ribosomes
engaged in protein synthesis. The proteins made on these ribosomes are
transported
into the space between the inner and outer nuclear membranes (the perinuclear space), which is continuous with the ER lumen (see Figure 12-9).
Bidirectional traffic occurs continuously between the cytosol and the nucleus. The many proteins that function in the nucleus - including histones, DNA and RNA polymerases, gene regulatory proteins, and RNA-processing proteins - are selectively imported into the nuclear compartment from the cytosol where they are made. At the same time, tRNAs and mRNAs are synthesized in the nuclear compartment and then exported to the cytosol. Like the import process, the export process is selective; mRNAs, for example, are exported only after they have been properly modified by RNA-processing reactions in the nucleus. In some cases the transport process is complex: ribosomal proteins, for instance, are made in the cytosol, imported into the nucleus - where they assemble with newly made ribosomal RNA into particles - and then exported again to the cytosol as part of a ribosomal subunit; each of these steps involves selective transport across the nuclear envelope.
(A) A sketch showing a small region of the nuclear envelope. In cross-section the nuclear pore complex appears composed of three parts: (1) a column component which forms the bulk of the pore wall; (2) an annular component, which extends "spokes" toward the center of the pore; and (3) a luminal component, which is formed by a large transmembrane glycoprotein that is thought to help anchor the complex to the nuclear membrane. In addition, fibrils protrude from both the cytosolic and nuclear sides of the complex. On the nuclear side the fibrils converge to form cagelike structures, which are shown in a scanning electron micrograph of the nuclear side of the nuclear envelope of an oocyte in (B). (B, from M.W. Goldberg and T.D. Allen, J. Cell Biol. 119:1429-1440, 1992, by copyright permission of the Rockefeller University Press.)
(A) and (B) Negatively stained views of nuclear pore complexes released from the envelope by detergent. In (B) some nuclear pore complexes can be seen on their side. (C) Three-dimensional computer reconstructions showing top, tilted, and side views of pore complexes. (From J.E. Hinshaw and R. Milligan, Cell 69:1133-1141, 1992. © Cell Press.)
and 12-11).
); this would mean that passive
diffusion and active
transport take place through different parts of the pore complex.
).
Because many cellular proteins are too large to pass by diffusion through the nuclear pores, the nuclear envelope allows the nuclear compartment and the cytosol to maintain different complements of proteins. Mature cytosolic ribosomes, for example, are about 30 nm in diameter and thus cannot diffuse through the 9-nm channels; their exclusion from the nucleus ensures that all protein synthesis is confined to the cytosol. But how does the nucleus export newly made ribosomal subunits or import large molecules, such as DNA and RNA polymerases, which have subunit molecular weights of 100,000 to 200,000? As we discuss next, these and many other protein and RNA molecules bind to specific receptor proteins located in the pore complexes and are then actively transported across the nuclear envelope through the complexes.
In general, the more active the nucleus is in transcription, the greater the number of pore complexes its envelope contains. The nuclear envelope of a typical mammalian cell contains 3000 to 4000 pore complexes. If the cell is synthesizing DNA, it needs to import about 10 6 histone molecules from the cytosol every 3 minutes in order to package newly made DNA into chromatin, which means that, on average, each pore complex needs to transport about 100 histone molecules per minute. If the cell is growing rapidly, each pore complex also needs to transport about 6 newly assembled large and small ribosomal subunits per minute from the nucleus, where they are produced, to the cytosol, where they are used. And that is only a very small part of the total traffic that passes through the nuclear pores.
When proteins are experimentally extracted from the nucleus and micro-injected back into the cytosol, even the very large ones efficiently reaccumulate in the nucleus. The selectivity of this nuclear protein import resides in nuclear localization signals, which are present only in nuclear proteins. The signals have been precisely defined in many nuclear proteins using recombinant DNA technology. They can be located almost anywhere in the amino acid sequence and generally consist of a short sequence (typically from four to eight amino acids) that varies for different nuclear proteins but is rich in the positively charged amino acids lysine and arginine and usually contains proline. In many nuclear proteins this sequence is split into two blocks of two to four amino acids each, with the blocks separated from each other by about ten amino acids. The signals are thought to form loops on the protein surface.
Immunofluorescence micrographs showing the cellular location of SV40 virus T-antigen containing or lacking a short peptide that serves as a nuclear localization signal. The wild-type T-antigen protein contains the lysine-rich sequence indicated and is imported to its site of action in the nucleus, as indicated by immunofluorescence staining with antibody against the T-antigen (A). T-antigen with an altered nuclear localization signal (a threonine replacing a lysine) remains in the cytosol (B). (From D. Kalderon, B. Roberts, W. Richardson, and A. Smith, Cell 39:499-509, 1984. © Cell Press.)
). On the
assumption that this mutation is in a nuclear localization signal sequence,
short
lengths of the DNA encoding this region of the normal T-antigen were fused
to a
gene coding for a cytosolic protein. The shortest sequence that caused the
resulting fusion protein to be imported into the nucleus encoded a stretch
of eight
contiguous amino acids, which is normally located in an internal region of the
T-antigen polypeptide chain (see Figure 12-13).
Further experiments showed
that the signal sequence could function even when it was linked as a short
peptide to selected lysine side chains on the surface of a cytosolic
protein, suggesting
that the precise location of a nuclear localization signal within the amino
acid
sequence of a nuclear protein is not important. In fact, many nuclear
proteins contain more than one nuclear localization signal.
).
) entering the
nucleus by means of
nuclear pores (indicated by red brackets). The same result is
obtained when
the gold spheres are coated with the tail regions of nucleoplasmin
molecules. These gold particles are much larger in diameter than the diffusion
channel in the pore complex, implying that a pore has been induced to widen
to permit their passage. Because the gold particles line up in the
cytosol before they contact and enter the pore complex, it has been suggested
that the fibrils that extend into the cytosol from the pore complex (see Figure 12-10A) guide the particles to their
destination (From C. Feldherr,
E. Kallenbach, and N. Schultz, J. Cell
Biol. 99:2216-2222, 1984, by copyright permission of the Rockefeller
University Press.)
and 12-15).
The proteins and structures involved in the active transport process are not known. A diverse set of related cytosolic proteins, however, is required for the initial binding of nuclear proteins to the complex. These proteins, called nucleoporins, contain a simple sugar ( N-acetylglucosamine) that aided their identification through the use of lectins and specific antibodies. The fibrils that project from the pore complex and are thought to help guide nuclear proteins to the center of the pore are not shown.
). Studies with various sizes of gold beads
indicate that the opening can
dilate up to about 26 nm in diameter during the transport process: a poorly
defined structure in the center of the nuclear pore complex appears to
function like
a close-fitting diaphragm that opens just the right amount when activated by
a signal on an appropriate large protein (see Figure 12-12). The molecular basis
of this mechanism, and how it operates to pump macromolecules both into and
out of the nucleus, is a mystery.
, are coated with
small RNA molecules (tRNA or 5S
RNA) and then injected into the nucleus of a frog oocyte, they are rapidly
transported through the nuclear pores into the cytosol. If they are
injected into the
cytosol of the oocyte, on the other hand, they remain there. Thus
it seems that, in
addition to receptors that recognize nuclear protein import signals, the pore
contains one or more receptors that recognize RNA molecules (or the proteins
bound to them) destined for the cytosol. Using differently sized gold
particles, one
set coated with RNA and injected into the nucleus and the other set coated
with nuclear protein import signals, it can be shown that a single pore
complex
allows traffic in both directions.
The mechanism of macromolecular transport across nuclear pores is fundamentally different from the transport mechanisms involved in the transfer of proteins across the membranes of other organelles in that it occurs through a large, regulated aqueous pore rather than through a protein transporter that spans one or more lipid bilayers. It is thought that a nuclear protein is transported through the pores while it is in a fully folded conformation, just as a newly formed ribosomal subunit is transported as an assembled particle; by contrast, proteins have to be unfolded during their transport into other organelles, as we discuss later.
Electron micrograph of a portion of the nuclear lamina in a Xenopus oocyte prepared by freeze drying and metal shadowing. The lamina is formed by a regular lattice of specialized intermediate filaments. (Courtesy of Ueli Aebi.)
). The nuclear lamina is thought to give
shape and stability to the nuclear
envelope, to which it is anchored by attachment to both the nuclear pore
complexes and the inner nuclear membrane. As the chromatin is also thought to
interact directly with the nuclear lamina, the lamina provides a structural
link
between the DNA and the nuclear envelope.
The phosphorylation of the lamins is thought to help trigger the disassembly of the nuclear lamina, which in turn causes the nuclear envelope to break up into vesicles. Dephosphorylation of the lamins is thought to help reverse the process.
). Because the
new nuclear envelope is so closely applied to the surface of the
chromosomes, it
excludes all of the proteins in the cell except those bound to the mitotic
chromosomes. Thus large proteins are kept out of the interphase nucleus unless
they contain nuclear localization signals.
Nuclear localization signals are not cleaved off after transport into the nucleus. This is presumably because nuclear proteins need to be imported repeatedly, once after every cell division. In contrast, once a protein molecule has been imported into any of the other membrane-bounded organelles, it is passed on from generation to generation within that compartment and need never be translocated again; the signal peptide on these molecules is often removed following protein translocation.
The glucocorticoid receptor is a gene regulatory protein that, in the non-hormone-treated cell, is bound in the cytosol to the chaperone protein hsp90. When activated by the binding of the appropriate steroid hormone, it is released from hsp90 and is directed into the nucleus by a nuclear localization signal; once in the nucleus, it binds to specific DNA sequences and regulates the transcription of a discrete set of genes (discussed in Chapters 9 and 15).
).
Export of RNA from the nucleus may be controlled in a similar way. Like active import into the nucleus, export also requires a signal: in the case of most messenger RNA molecules, this is provided by a unique modification, the cap structure, at the 5' end of the RNA (discussed in Chapter 8). Incompletely processed pre-messenger RNAs include this cap but are anchored to the nuclear transcription and splicing machinery, which releases an RNA molecule only after its processing is completed: genetic studies in yeast have shown that mutations that prevent the pre-messenger RNA from properly engaging with the splicing machinery lead to the export of the unspliced RNA. Other RNAs, like transfer RNA or ribosomal RNA, which lack a 5' cap, must first be assembled with proteins and are then exported as part of these complexes. Presumably, nuclear export signals are contained in the protein subunits of these complexes, and these signals become activated after proper assembly with the RNA components, but the nature of these signals is not known.
The nuclear envelope consists of an inner and an outer nuclear membrane. The outer membrane is continuous with the ER membrane, and the space between it and the inner membrane is continuous with the ER lumen. RNA molecules, which are made in the nucleus, and ribosomal subunits, which are assembled there, are exported to the cytosol, while all of the proteins that function in the nucleus are synthesized in the cytosol and are then imported. The extensive traffic of materials between nucleus and cytosol occurs through nuclear pores that provide a direct passageway across the nuclear envelope.
Proteins containing nuclear localization signals are actively transported inward through the pores, while RNA molecules and newly made ribosomal subunits are actively transported outward through the pores. Because the nuclear localization signals are not removed, nuclear proteins can be imported repeatedly, as is required each time the nucleus reassembles following mitosis. The transport of nuclear proteins and RNA molecules through the pores can be regulated by denying these molecules access to the transport machinery in the nuclear pore complexes.
The topology of the chloroplast can be derived from that of the mitochondrion in a simple way: pinching off the invaginations of the inner mitochondrial membrane to create vesicles would generate a compartment that is topologically equivalent to the thylakoid vesicle in chloroplasts. Thylakoid vesicles may have evolved in this way.
). Chloroplasts have
the same two subcompartments plus an additional subcompartment, the thylakoid space, which is surrounded by the thylakoid membrane ( Figure 12-20B). Each
of the subcompartments contains a distinct set of proteins. The growth of
mitochondria and chloroplasts by the import of proteins from the cytosol is
therefore a major feat, requiring that proteins be translocated across a
number of
membranes in succession and end up in the appropriate place.
The relatively few proteins encoded by the genomes of these organelles are located mostly in the inner membrane in mitochondria and in the thylakoid membrane in chloroplasts. These organelle-encoded polypeptides generally form subunits of protein complexes whose other subunits are encoded by nuclear genes and are imported from the cytosol. The formation of such hybrid protein complexes requires a balanced synthesis of the two types of subunits; how protein synthesis is coordinated on different types of ribosomes located two membranes apart is still largely a mystery.
Cytochrome oxidase is a large multiprotein complex located in the mitochondrial inner membrane, where it functions as the terminal enzyme in the electron-transport chain (discussed in Chapter 14). (A) The first 12 amino acids of the precursor to subunit IV of this enzyme serve as a signal peptide for the import of the subunit into the mitochondrion. (B) When the full-length signal peptide is folded as an alpha helix with 3.6 residues per turn and viewed from the top, the positively charged residues ( red) are seen to be clustered on one face of the helix while the nonpolar residues ( green) are clustered on the opposite face. Mitochondrial signal peptide sequences always have the potential to form such an amphipathic helix, which is thought to be recognized by specific receptor proteins on the mitochondrial surface.
). This configuration is thought
to be recognized by specific
receptor proteins on the mitochondrial surface.Almost everything we know about the molecular mechanism of protein import into mitochondria has been learned from analysis of cell-free, reconstituted transport systems. Mitochondria are first purified by differential centrifugation of homogenized cells and are then incubated with radiolabeled mitochondrial precursor proteins. The precursor proteins are generally taken up rapidly and efficiently into such mitochondria during a brief in vitro incubation. By changing the conditions in these experiments in vitro, it is possible to establish the biochemical requirements for protein transport into the mitochondria.
Vectorial movement and transport require energy. In most biological systems the energy is supplied by ATP hydrolysis. In the case of mitochondrial import, however, an electrochemical gradient across the inner mitochondrial membrane is required in addition to ATP hydrolysis. This gradient is maintained by the pumping of H + from the matrix to the intermembrane space, driven by electron transport processes in the inner membrane. The mitochondrial outer membrane, like that of gram-negative bacteria (see Figure 11-14), contains large amounts of a pore-forming protein called porin and is thus freely permeable to inorganic ions and metabolites (but not to most proteins), so that no gradient can be maintained across it. The energy in the electrochemical gradient across the inner membrane is tapped to help drive most of the cell's ATP synthesis, but it is also used to drive the translocation of proteins bearing a mitochondrial import signal peptide: when ionophores that collapse the mitochondrial membrane potential are added, import is blocked. It is still uncertain how the electrochemical gradient contributes to protein translocation. The role of ATP hydrolysis is much better understood, as we see below.
As a first step in mitochondrial import, the mitochondrial precursor proteins have to bind to receptor proteins that reside in the mitochondrial outer membrane and recognize the mitochondrial signal peptides. The next step is the translocation process itself.
When isolated mitochondria are incubated with a precursor protein at 5°C, the precursor is only partially translocated. The amino-terminal signal peptide ( red) is cleaved off in the matrix; most of the polypeptide chain remains outside the mitochondria, where it is accessible to proteolytic enzymes. Upon warming to 25°C, the translocation is completed. Once inside the mitochondrion, the polypeptide chain is protected from externally added proteolytic enzymes unless detergents are added to disrupt the mitochondrial membranes, which allows the imported proteins to be digested.
). This result demonstrates that the
precursor proteins can pass
through both mitochondrial membranes at once to enter the matrix. It is
thought
that there are two protein translocators, one in the outer membrane and one in
the inner membrane, whose functions are usually coupled to allow
translocation across both membranes at the same time. Electron
microscopists have
noted numerous contact sites at which the inner and outer mitochondrial
membranes appear to be joined, and it seems likely that translocation
occurs at or near
these sites.
The amino-terminal signal peptide of the precursor protein is recognized by receptors that reside in the outer membrane. The protein is thought to be translocated across both mitochondrial membranes at or near special contact sites, driven first by the electrochemical gradient across the inner membrane and then by ATP hydrolysis. The signal peptide is cleaved off by a signal peptidase in the matrix to form the mature protein; the free signal peptide is rapidly degraded.
that the
import process occurs in two distinct stages, only the second of which is
arrested at
a low temperature. Of these, it is only the initial penetration, which is not
affected by low temperatures, that requires the membrane potential: when
cooled
mitochondria containing partly translocated intermediates are warmed up,
import
is rapidly completed (see Figure 12-22) even if
the potential across the inner
membrane is collapsed. This second stage of the transport process, however,
requires ATP. Thus the first stage, which involves the insertion of
the signal peptide
and adjoining sequences into both mitochondrial membranes, is driven by the
electrochemical gradient, and the second stage, in which the remainder of the
polypeptide chain moves into the matrix, requires both ATP hydrolysis and a
physiological temperature ( Figure 12-23).Transport of mitochondrial precursor proteins across the two mitochondrial membranes at a contact site is guided by members of the chaperone family of proteins, which are discussed in Chapter 5. It is difficult to envisage how a folded, water-soluble protein could straddle two (or even one) lipid bilayer while retaining its native three-dimensional conformation. It is now known that cytosolic chaperone proteins (called chaperonins) belonging to the hsp70 family, as well as helping to ensure the correct folding of cytosolic proteins, play an essential part in protein import into both mitochondria and the ER by binding the precursor in its unfolded state during translocation. As discussed in Chapter 5, the release of newly synthesized polypeptides from the hsp70 family of chaperone proteins requires ATP hydrolysis, and this partly accounts for the ATP dependence of the later stages of mitochondrial import.
The essential role of the chaperone proteins in translocation across internal cellular membranes was first indicated by genetic studies in yeasts. When the genes encoding certain members of the hsp70 family of chaperone proteins are inactivated, mitochondrial precursor proteins fail to be imported into mitochondria and accumulate in the cytosol instead. It is thought that newly synthesized precursor proteins, as they are released from polyribosomes in the cytosol, bind to hsp70 proteins, which prevent the precursor proteins from aggregating or folding up spontaneously before they bind to the protein translocator in the target membrane. The energy liberated by the hydrolysis of ATP is used to release the bound hsp70 proteins as the translocated protein is passed across the membrane. Experimentally, the requirement for hsp70 and ATP in the cytosol can be bypassed if the precursor proteins are artificially unfolded, for example, by a denaturation step in a concentrated solution of urea.
After the initial insertion of the signal peptide and of adjacent portions of the polypeptide chain, the unfolded chain slides in a channel that spans both membranes. Bound cytosolic hsp70 is released from the protein in a step that depends on ATP hydrolysis; concomitantly, mitochondrial hsp70 binds to regions of the polypeptide chain as they become exposed in the matrix, thereby pulling the protein into the interior of the mitochondrion.
): the sequential
binding of multiple mitochondrial hsp70 proteins may pull the unfolded
protein through a transmembrane channel into the matrix.
After the initial interaction with mitochondrial hsp70, many imported proteins are passed on to another chaperone protein, mitochondrial hsp60. As discussed in Chapter 5, hsp60 attaches to the unfolded polypeptide chain and facilitates its folding in an ATP-consuming reaction. Much of our current understanding of the function of hsp60 in facilitating protein folding is derived from studies on import of proteins into mitochondria.
. Cleavage of
the signal peptide
( red) used for the initial translocation, however, unmasks an
adjacent hydrophobic signal peptide
( orange) at the new amino terminus. This signal causes the
protein to
be integrated into the inner membrane by the same pathway that is used
to insert proteins encoded by the mitochondrial genome into
this membrane. (B) In an alternative mechanism, the
hydrophobic sequence that follows the matrix targeting signal binds to
the translocator and stops the translocation across the
inner membrane. The remainder of the protein is then pulled into
the intermembrane space and the hydrophobic sequence is
released into the inner membrane. This mechanism is called the
stop-transfer pathway and is discussed in detail later. (C) Some soluble
proteins of
the intermembrane space may also use the pathways shown in (A) and
(B) before they are released into the intermembrane space by a
second signal peptidase (with its active site in the intermembrane space),
which removes the hydrophobic signal peptide.
.
A very hydrophobic amino acid sequence, however, is strategically placed after
the amino-terminal signal peptide that initiates import. Once the
amino-terminal signal is cleaved by the matrix signal peptidase, the
hydrophobic sequence
can function as a new amino-terminal signal peptide to translocate the protein
back again from the matrix into or across the inner membrane. Presumably, the
final step in this pathway involves a mechanism that is also used to direct
proteins encoded in the mitochondrion to the inner membrane ( Figure 12-25A), and
we see later that a similar mechanism is used for translocating proteins
into or
across the ER membrane and the procaryotic plasma membrane, where it has
been more extensively investigated.
). Different proteins may use
one or the other of these two
pathways to the inner membrane or intermembrane space. It is not clear which
one is more commonly used.
). Many of these proteins
ultimately become attached as peripheral membrane proteins to the outer
surface of
the inner membrane, where they form subunits of protein complexes that also
contain transmembrane proteins.Protein transport into chloroplasts resembles transport into mitochondria in many respects: both occur posttranslationally, both require energy, and both utilize amphipathic amino-terminal signal peptides that are removed after use. There is at least one important difference, however: mitochondria exploit the electrochemical gradient across their inner membrane to help drive the transport, whereas chloroplasts, which have an electrochemical gradient across their thylakoid but not their inner membrane, appear to employ only ATP hydrolysis to power import across their double-membrane outer envelope.
Although the signal peptides for import into chloroplasts resemble those for import into mitochondria, mitochondria and chloroplasts are both present in the same plant cells, and proteins must choose appropriately between them. In plants, for example, a bacterial enzyme is directed specifically to mitochondria if it is experimentally joined to an amino-terminal signal sequence of a mitochondrial protein; the same enzyme joined to an amino-terminal signal sequence of a chloroplast protein ends up in chloroplasts. The different signal sequences, therefore, can be distinguished, presumably by the import receptors on each organelle.
The precursor polypeptide contains an amino-terminal chloroplast signal peptide ( red) followed immediately by a thylakoid signal peptide ( orange). The chloroplast signal peptide initiates translocation into the stroma through a membrane contact site by a mechanism similar to that used for translocation into the mitochondrial matrix. The signal peptide is then cleaved off, unmasking the thylakoid signal peptide, which initiates translocation across the thylakoid membrane.
). As with
mitochondria, the second step is the pathway used to insert
chloroplast-encoded
proteins into the thylakoid membrane; the protein translocator required
presumably
originated in the chloroplast's bacterial ancestor.Although mitochondria and chloroplasts have their own genetic systems, they produce only a small proportion of their own proteins. Instead, the two organelles import most of their proteins from the cytosol using similar mechanisms. The transport processes involved have been most extensively studied in mitochondria, especially in yeasts. A protein is translocated into the mitochondrial matrix space by passing through sites of adhesion between the outer and inner membranes called contact sites. Translocation into mitochondria is driven by both ATP hydrolysis and the electrochemical gradient across the inner membrane, whereas translocation into chloroplasts is driven by ATP hydrolysis alone. The transported protein crosses the membranes of the mitochondrion or chloroplast in an unfolded state. Chaperone proteins of the cytosolic hsp70 family maintain the precursor proteins in an unfolded, translocation-competent state. Mitochondrial hsp70 in the matrix binds to the incoming polypeptide chain and is thought to pull the protein chain into the matrix. Once the protein is in the matrix, another stress protein, hsp60, helps the translocated protein fold up. Only proteins that contain a specific signal peptide are translocated into mitochondria or chloroplasts. The signal peptide is usually located at the amino terminus and is cleaved off after import. Transport across or into the inner membrane can occur as a second step if a hydrophobic signal peptide is also present in the imported protein; this second signal peptide is unmasked when the first signal peptide is removed. In the case of chloroplasts, import from the stroma into the thylakoid likewise requires a second signal peptide.
Peroxisomes differ from mitochondria and chloroplasts in many ways. Most notably, they are surrounded by only a single membrane, and they do not contain DNA or ribosomes. In spite of these differences, peroxisomes are thought to acquire their proteins by a similar process of selective import from the cytosol. Because peroxisomes have no genome, however, all of their proteins must be imported. Peroxisomes thus resemble the ER in being self-replicating membrane-bounded organelles that exist without genomes of their own.
Electron micrograph of three peroxisomes in a rat liver cell. The paracrystalline electron-dense inclusions are the enzyme urate oxidase. (Courtesy of Daniel S. Friend.)
).
Like the mitochondrion, the peroxisome is a major site of oxygen utilization. One hypothesis is that the peroxisome is a vestige of an ancient organelle that carried out all of the oxygen metabolism in the primitive ancestors of eucaryotic cells. When the oxygen produced by photosynthetic bacteria first began to accumulate in the atmosphere, it would have been highly toxic to most cells. Peroxisomes might have served to lower the intracellular concentration of oxygen while also exploiting its chemical reactivity to carry out useful oxidative reactions. According to this view, the later development of mitochondria rendered the peroxisome largely obsolete because many of the same reactions - which had formerly been carried out in peroxisomes without producing energy - were now coupled to ATP formation by means of oxidative phosphorylation. The oxidative reactions carried out by peroxisomes in present-day cells would therefore be those that have important functions not taken over by mitochondria.
Peroxisomes are so called because they usually contain one or more enzymes that use molecular oxygen to remove hydrogen atoms from specific organic substrates (designated here as R) in an oxidative reaction that produces hydrogen peroxide (H2O2):
Catalase utilizes the H2O2 generated by other enzymes in the organelle to oxidize a variety of other substrates - including phenols, formic acid, formaldehyde, and alcohol - by the "peroxidative" reaction: H2O2 + R'H2→ R' + 2H2O. This type of oxidative reaction is particularly important in liver and kidney cells, whose peroxisomes detoxify various toxic molecules that enter the bloodstream. About a quarter of the ethanol we drink is oxidized to acetaldehyde in this way. In addition, when excess H2O2 accumulates in the cell, catalase converts it to H2O (2H2O2→ 2H2O + O2).
A major function of the oxidative reactions carried out in peroxisomes is the breakdown of fatty acid molecules. In a process called β oxidation, the alkyl chains of fatty acids are shortened sequentially by blocks of two carbon atoms at a time that are converted to acetyl CoA and exported from the peroxisomes to the cytosol for reuse in biosynthetic reactions. β oxidation in mammalian cells occurs both in mitochondria and peroxisomes; in yeast and plant cells, however, this essential reaction is exclusively found in peroxisomes.
Peroxisomes are unusually diverse organelles and even in the different cells of a single organism may contain very different sets of enzymes. They also can adapt remarkably to changing conditions. Yeast cells grown on sugar, for example, have small peroxisomes. But when some yeasts are grown on methanol, they develop large peroxisomes that oxidize methanol; and when grown on fatty acids, they develop large peroxisomes that break down fatty acids to acetyl CoA by β oxidation.
(A) A leaf peroxisome with a paracrystalline core in a tobacco leaf mesophyll cell. Its close association with chloroplasts is thought to facilitate the exchange of materials between these organelles during photorespiration. (B) Peroxisomes in a fat-storing cotyledon cell of a tomato seed 4 days after germination. Here the peroxisomes ( glyoxysomes) are associated with the lipid bodies where fat is stored, reflecting their central role in fat mobilization and gluconeogenesis during seed germination. (A, courtesy of P.J. Gruber and E.H. Newcomb; B, courtesy of S.E. Frederick and E.H. Newcomb.)
). This process is called photorespiration because it uses up
O 2 and liberates CO 2. The other type of
peroxisome is present in
germinating seeds, where it plays an essential role in converting the fatty
acids stored in
seed lipids into the sugars needed for the growth of the young plant. Because
this conversion of fats to sugars is accomplished by a series of reactions
known as
the glyoxylate cycle, these peroxisomes are also called glyoxysomes ( Figure 12-28B). In the
glyoxylate cycle two molecules of acetyl CoA produced by fatty acid
breakdown in the peroxisome are used to make succinic acid, which leaves the
peroxisome and is converted into glucose. The glyoxylate cycle does not occur
in animal cells, and animals are thus unable to convert the fatty acids in
fats
into carbohydrates.
The peroxisome membrane contains specific import receptor proteins. All peroxisomal proteins, including new copies of the import receptor, are synthesized by cytosolic ribosomes and then imported into the organelle. Thus peroxisomes form only from preexisting peroxisomes by a process of growth and fission. Presumably, the lipids required to make new peroxisome membrane are also imported. We discuss later how lipids made in the ER can be transported through the cytosol to other organelles.
).Peroxisomes are specialized for carrying out oxidative reactions using molecular oxygen. They generate hydrogen peroxide, which they also use for oxidative purposes - destroying the excess by means of the catalase they contain. Like mitochondria and plastids, peroxisomes are self-replicating organelles. Because they contain no DNA or ribosomes, they have to import all of their proteins from the cytosol. A specific three amino acid sequence near the carboxyl terminus of many of these proteins functions as a peroxisomal import signal.
Fluorescence micrograph of a cultured mammalian cell stained with an antibody that binds to a protein retained in the ER. The ER extends as a network throughout the entire cytosol, so that all regions of the cytosol are close to some portion of the ER membrane. (Courtesy of Hugh Pelham.)
). The tubules and
sacs are all thought to interconnect, so that the ER membrane forms a
continuous sheet enclosing a single internal space. This highly convoluted
space is called
the ER lumen or the ER cisternal space, and it often occupies
more than 10% of
the total cell volume (see Table 12-1). The ER
membrane separates the ER
lumen from the cytosol, and it mediates the selective transfer of molecules
between these two compartments.
The ER plays a central part in lipid and protein biosynthesis. Its membrane is the site of production of all the transmembrane proteins and lipids for most of the cell's organelles, including the ER itself, the Golgi apparatus, lysosomes, endosomes, secretory vesicles, and the plasma membrane. The ER membrane also makes a major contribution to mitochondrial and peroxisomal membranes by producing most of their lipids. In addition, almost all of the proteins that will be secreted to the cell exterior - as well as those destined for the lumen of the ER, Golgi apparatus, or lysosomes - are initially delivered to the ER lumen.
The ER captures selected proteins from the cytosol as they are being synthesized. These proteins are of two types: (1) transmembrane proteins, which are only partly translocated across the ER membrane and become embedded in it, and (2) water-soluble proteins, which are fully translocated across the ER membrane and are released into the ER lumen. Some of the transmembrane proteins will remain in the ER, but many are destined to reside in the plasma membrane or the membrane of another organelle; the water-soluble proteins are destined either for the lumen of an organelle or for secretion. All of these proteins, regardless of their subsequent fate, are directed to the ER membrane by the same kind of signal peptide and are translocated across it by the same mechanism.
Electron micrograph of the rough ER, which receives its name from the many ribosomes on its cytosolic surface. (Courtesy of L. Orci.)
).
Thin-section electron micrograph of polyribosomes attached to the ER membrane. The plane of section in some places cuts through the ER roughly parallel to the membrane, giving a face-on view of the rosettelike pattern of the polyribosomes. (Courtesy of George Palade.)
A common pool of ribosomes is used to synthesize both the proteins that stay in the cytosol and those that are transported into the ER. It is the ER signal peptide on a newly formed polypeptide chain that directs the engaged ribosome to the ER membrane. The mRNA molecule may remain permanently bound to the ER as part of a polyribosome, while the ribosomes that move along it are recycled; at the end of each round of protein synthesis, the ribosomal subunits are released and rejoin the common pool in the cytosol.
). The individual ribosomes associated with
such an mRNA molecule can return
to the cytosol when they finish translation near the
3' end of the mRNA molecule. The mRNA itself, however, tends to remain
attached to the ER membrane by
a changing population of ribosomes that are also held at the membrane by a
ribosome receptor that helps to bind it there. In contrast, if an mRNA
molecule
encodes a protein that lacks an ER signal peptide, the polyribosome that
forms remains free in the cytosol and its protein product is discharged there.
Therefore, only those mRNA molecules that encode proteins with an ER signal
peptide
bind to rough ER membranes; those mRNA molecules that encode all other
proteins remain free in the cytosol. The individual ribosomal subunits are
thought to move randomly between these two segregated populations of mRNA
molecules
( Figure 12-33).
This electron micrograph is of a testosterone-secreting Leydig cell in the human testis.
).
The rough ER forms oriented stacks of flattened cisternae, each having a luminal space 20 to 30 nm wide. The smooth ER membrane is connected to these cisternae and forms a fine network of tubules 30 to 60 nm in diameter. (After R.V. Krstić Ultrastructure of the Mammalian Cell. New York: Springer-Verlag, 1979.)
and
see Table 12-2).
When large quantities of certain compounds, such as the drug phenobarbital, enter the circulation, detoxification enzymes are synthesized in the liver in unusually large amounts, and the smooth ER doubles in surface area within a few days. Once the drug disappears, the excess smooth ER membrane is specifically and rapidly removed by a lysosome-dependent process called autophagocytosis (discussed in Chapter 13). How these dramatic changes are regulated is not known.
Another function of the ER in most eucaryotic cells is to sequester Ca 2+ from the cytosol. The release of Ca 2+ into the cytosol from the ER, and its subsequent reuptake, mediate many rapid responses to extracellular signals, as discussed in Chapter 15. The storage of Ca 2+ in the ER lumen is facilitated by the high concentrations of Ca 2+-binding proteins there. In some cell types, and perhaps in most, specific regions of the ER are specialized for Ca 2+ storage. Muscle cells, for example, have an abundant specialized smooth ER, called the sarcoplasmic reticulum, which sequesters Ca 2+ from the cytosol by means of a Ca 2+-ATPase that pumps in Ca 2+; the release and reuptake of Ca 2+ by the sarcoplasmic reticulum mediates the contraction and relaxation of the myofibrils during each round of muscle contraction (discussed in Chapter 16).
We shall now return to the two major roles of the ER: the synthesis and modification of proteins and the synthesis of lipids.
When cells are disrupted by homogenization, the cisternae of rough ER (A) break up into small closed vesicles called rough microsomes (B). Similarly, the smooth ER breaks up into small vesicles that lack ribosomes and are called smooth microsomes. (A, courtesy of Daniel S. Friend; B, courtesy of George Palade.)
). Because they
can be readily purified in functional form, rough microsomes are especially
useful
for studying the many processes carried out by the rough ER. To the biochemist
they represent small authentic versions of the rough ER, still capable of
protein
synthesis, protein glycosylation, and lipid synthesis.
Many vesicles of a size similar to that of rough microsomes but lacking attached ribosomes are also found in these homogenates. Such smooth microsomes are derived in part from smooth portions of the ER and in part from vesiculated fragments of plasma membrane, Golgi apparatus, endosomes, and mitochondria (the ratio depending on the tissue). Thus, whereas rough microsomes can be equated with rough portions of ER, the origins of smooth microsomes cannot be so easily assigned. The microsomes of the liver are an exception. Because of the unusually large quantities of smooth ER in the hepatocyte, most of the smooth microsomes in liver homogenates are derived from smooth ER.
When sedimented to equilibrium through a gradient of sucrose, the two types of microsomes separate from each other on the basis of their different densities.
). When
the separated rough and smooth microsomes of liver are compared with respect
to such properties as enzyme activity or polypeptide composition, they are
very similar, although not identical: apparently most of the components of the
ER membrane can diffuse freely between the rough and smooth regions, as
would be expected for a continuous fluid membrane. The rough microsomes,
however, contain more than 20 proteins that are not present in smooth
microsomes,
showing that some restraining mechanism must exist for a subset of ER
membrane proteins. Some of the proteins in this subset help bind ribosomes
to the
rough ER, while others presumably produce the flattened shape of this part
of the
ER (see Figure 12-35). It is not clear whether
these membrane proteins are
retained by forming large two-dimensional aggregates in the lipid bilayer
or whether
they are instead held in place by interactions with a network of structural
proteins
on one or the other face of the ER membrane.
A simplified view of protein translocation across the ER membrane, as originally proposed. When the signal peptide emerges from the ribosome, it directs the ribosome to a receptor protein on the ER membrane. As it is synthesized, the polypeptide is postulated to be translocated across the ER membrane through a protein pore associated with the receptor. The signal peptide is clipped off during translation by a signal peptidase, and the mature protein is released into the lumen of the ER immediately after being synthesized. We now know that the hypothesis is correct in outline but that additional components besides those shown in this figure are required. The signal peptidase, for example, is a complex of five different membrane-bound polypeptide chains, with one complex apparently associated with every translocation pore.
).
According to the signal hypothesis, the secreted protein should be extruded into the lumen of the microsome during its in vitro synthesis. This can be demonstrated with protease treatment: a newly synthesized protein made in the absence of microsomes is degraded when protease is added to the medium, whereas the same protein made in the presence of microsomes remains intact because it is protected by the microsomal membrane. When proteins without ER signal peptides are similarly synthesized in vitro,they are not imported into microsomes and therefore are degraded by protease treatment.
The signal hypothesis has been thoroughly tested by genetic and biochemical experiments and is found to apply to both plant and animal cells, as well as to protein translocation across the bacterial plasma membrane and, as we have seen, the membranes of mitochondria, chloroplasts, and peroxisomes. Amino-terminal ER signal peptides guide not only secreted proteins but also the precursors of all proteins made in the ER, including soluble proteins and membrane proteins. The signaling function of these peptides has been demonstrated directly by using recombinant DNA techniques to attach signal sequences to proteins that do not normally have them; the resulting fusion proteins are directed to the ER.
Cell-free systems in which proteins are imported into microsomes have provided powerful assay procedures for identifying, purifying, and studying the various components of the molecular machinery responsible for the ER import process.
An SRP is an elongated complex containing six protein subunits and one RNA molecule (SRP RNA). One end of the SRP binds to an ER signal peptide on a growing polypeptide chain, while the other end binds to the ribosome itself and stops translation. The RNA in the particle may mediate an interaction with ribosomal RNA. (Adapted from V. Siegel and P. Walter, Nature 320:82-84, 1986.)
). SRP and
SRP receptor are present in all eucaryotic cells and probably in
procaryotic cells
as well.
The SRP binds to the ER signal peptide as soon as the peptide emerges from the ribosome. This causes a pause in protein synthesis, which presumably gives the ribosome enough time to bind to the ER membrane before the synthesis of the polypeptide chain is completed, thereby ensuring that the protein is not released into the cytosol. This may provide a safety mechanism as many secreted proteins and lysosomal proteins are hydrolases that could wreak havoc in the cytosol. Cells that secrete large amounts of hydrolases take the added precaution of having high concentrations of hydrolase inhibitors in their cytosol.
The SRP and the SRP receptor are thought to act in concert. The SRP binds to the exposed ER signal peptide and to the ribosome, thereby inducing a pause in translation. The SRP receptor in the ER membrane, which is composed of two different polypeptide chains, binds the SRP ribosome complex. In a poorly understood reaction that involves multiple GTP-binding proteins, the SRP is released, leaving the ribosome on the ER membrane. A multisubunit protein translocation apparatus in the ER membrane then inserts the polypeptide chain into the membrane and transfers it across the lipid bilayer.
). Because one of the SRP
proteins and both chains of the SRP
receptor contain GTP-binding domains, it is thought that conformational
changes that occur during cycles of GTP binding and hydrolysis (discussed
in Chapter
5) ensure that SRP release occurs only after the ribosome has become
properly engaged with the translocation apparatus in the ER membrane.
In this schematic model, after a receptor in the translocation complex has bound the amino-terminal signal peptide, an energy-driven protein translocator threads the protein through the membrane, unfolding the polypeptide chain in the process. The energy is provided both by ATP hydrolysis and an electrochemical gradient across the membrane.
). In
both cases the translocation requires ATP hydrolysis, and in bacteria an
electrochemical gradient is needed as well. A translocation apparatus has been
reconstituted from purified bacterial components, one of which is an ATPase
that is
thought to help thread the protein through the membrane ( Figure 12-41). Since the
proteins that use a posttranslational translocation pathway are first
released into
the cytosol, they are prevented from folding up by binding to cytosolic
chaperone proteins, just as we have seen for the posttranslational import into
mitochondria and chloroplasts.
The experimental set-up is similar to that shown in Figure 10-5, with an artificial lipid bilayer separating two aqueous compartments. When rough microsomes are added to one of the compartments, they occasionally fuse with the lipid bilayer, incorporating a portion of ER membrane (with its bound ribosomes) into the bilayer. When the drug puromycin ( dark blue) is added to the same compartment, it couples covalently to the carboxyl terminus of the growing polypeptide chain and releases it from the ribosome; pores of uniform size can now be detected as discrete increases in the electrical conductance across the membrane (the ion flow responsible for the increased electrical conductance is indicated by the yellow arrow). If the ribosomes are removed from the membrane with a high-salt wash, pores are no longer detected, indicating that ribosome binding is required to open (or assemble) the pore (not shown).
). Thus the
pore seems to be a dynamic structure, opening when a ribosome with a
growing polypeptide chain attaches to the membrane and closing when the
ribosome detaches after the synthesis of the protein is completed.We have seen that in chloroplasts and mitochondria the signal peptides are cleaved from the precursor proteins once they have crossed the membrane. Similarly, amino-terminal ER signal peptides are removed by a signal peptidase on the luminal side of the ER membrane. The peptide by itself, however, is not sufficient to signal cleavage by the peptidase; this requires an adjacent cleavage site that is specifically recognized by the peptidase. We shall see below that ER signal peptides that are contained within the polypeptide chain rather than at the amino terminus do not have these recognition sites and are never cleaved; instead, they can serve to retain transmembrane proteins in the lipid bilayer after the translocation process has been completed.
). After the protein
has been completely translocated, the translocator reverts to an
inactive conformation, which can no longer conduct ions across the
membrane but is open to the lipid bilayer, allowing the hydrophobic
signal peptide to diffuse out into the bilayer, where it is rapidly
degraded. In
this and the following two figures the ribosomes have been omitted
for clarity.
).The translocation process for proteins destined to remain in the membrane is more complex than it is for soluble proteins, as some parts of the polypeptide chain are translocated across the lipid bilayer whereas others are not. Nevertheless, all modes of insertion of membrane proteins can be considered as variants of the sequence of events just described for transferring a soluble protein into the lumen of the ER. We begin by describing the three ways in which single-pass transmembrane proteins (see Figure 10-13) become inserted into the ER.
. In addition to the
start-transfer peptide,
however, the protein also contains a stop-transfer peptide
( orange). When the stop-transfer peptide enters
the translocator and interacts with a binding site, the translocator
flips into its inactive state and discharges the protein laterally
into the lipid bilayer.
). The
stop-transfer peptide forms a single
alpha-helical membrane-spanning segment, with the amino terminus of the
protein on
the luminal side of the membrane and the carboxyl terminus on the cytosolic
side.
and that shown in (B) here.
), while in the other it has its
amino terminus on the luminal side ( Figure 12-45B). The orientation of the
start-transfer peptide depends on the distribution of nearby charged amino
acids, as
described in the figure legend.
) and initiates
the transfer of the carboxyl terminal arm of the polypeptide chain. When
a stop-transfer peptide enters the translocator, it discharges the
protein laterally into the membrane.
Rhodopsin is the light-sensitive protein in rod photoreceptor cells in the mammalian retina. (A) A hydrophobicity plot identifies seven short hydrophobic regions in rhodopsin. (B) The most amino-terminal region serves as a start-transfer peptide that causes the preceding amino-terminal portion of the protein to be passed across the ER membrane. Subsequent hydrophobic peptides will function in alternation as start-transfer and stop-transfer peptides. (C) The final integrated rhodopsin has its amino terminus located in the ER lumen and its carboxyl terminus located in the cytosol. The blue hexagonsrepresent covalently attached oligosaccharides.
). In more
complex multipass proteins, in
which many hydrophobic alpha helices span the bilayer, a second start-transfer
peptide reinitiates translocation further down the polypeptide chain until
the next
stop-transfer peptide causes polypeptide release, and so on for subsequent
start-transfer and stop-transfer peptides ( Figure 12-47).
Whether a given hydrophobic signal sequence will function as a start-transfer or stop-transfer peptide must depend on its location in a polypeptide chain, since its function can be switched by changing its location in the protein using recombinant DNA techniques. Thus the distinction between start-transfer and stop-transfer peptides results mostly from their relative order in the growing polypeptide chain. It seems that the SRP begins scanning an unfolded polypeptide chain for hydrophobic segments at its amino terminus and proceeds toward the carboxyl terminus, in the direction that the protein is synthesized. By recognizing the first appropriate hydrophobic segment to emerge from the ribosome, the SRP sets the "reading frame": if translocation is initiated, the next appropriate hydrophobic segment will be recognized as a stop-transfer peptide, causing the region of the polypeptide chain in between to be threaded across the membrane. A similar scanning process continues until all of the hydrophobic regions in the protein have been inserted into the membrane.
Because membrane proteins are always inserted from the cytosolic side of the ER in this programmed manner, all copies of the same polypeptide chain will have the same orientation in the lipid bilayer. This generates an asymmetrical ER membrane in which the protein domains exposed on one side are different from those domains exposed on the other. This asymmetry is maintained during the many membrane budding and fusion events that transport the proteins made in the ER to other cell membranes (discussed in Chapter 13). Thus the way in which a newly synthesized protein is inserted into the ER membrane determines the orientation of the protein in the other membranes as well.
When proteins are dissociated from a membrane and reconstituted in artificial lipid vesicles, a random mixture of right-side-out and inside-out protein orientations usually results. Thus the protein asymmetry observed in cell membranes seems not to be an inherent property of the protein but to result solely from the process by which proteins are inserted into the ER membrane from the cytosol.
Another ER resident protein is a chaperone protein known as binding protein (BiP), which is structurally related to the hsp70 proteins and, like them, recognizes incorrectly folded proteins, as well as protein subunits that have not yet assembled into their final oligomeric complexes. BiP, like other chaperone proteins, is thought to bind to exposed amino acid sequences that would normally be buried in the interior of correctly folded or assembled polypeptide chains. The bound BiP both prevents the proteins from aggregating and helps to keep them in the ER (and thus out of the Golgi apparatus and later parts of the secretory pathway); it may also help them to fold normally. Like the hsp70 family of proteins, which bind unfolded proteins in the cytosol and facilitate their import into mitochondria and chloroplasts, BiP hydrolyzes ATP to provide the energy for its role in protein folding.
), the
binding of BiP to an unfolded protein chain emerging in the ER lumen may help
pull the protein into the ER. This pulling process may be particularly
important
for proteins that enter the ER posttranslationally because in this case
there is no
ribosome attached to the membrane to help push the nascent protein through
the translocator during the protein's synthesis.The covalent addition of sugars to proteins is one of the major biosynthetic functions of the ER. Most of the soluble and membrane-bound proteins that are made in the ER, including those destined for transport to the Golgi apparatus, lysosomes, plasma membrane, or extracellular space are glycoproteins. In contrast, very few proteins in the cytosol are glycosylated, and those that are carry a much simpler sugar modification in which a single N-acetylglucosamine group is added to a serine or threonine residue of the protein.
The five sugar residues in the gray box form the "core region" of this oligosaccharide. For many glycoproteins only the core sugars survive the extensive oligosaccharide trimming process that takes place in the Golgi apparatus. Only asparagines in the sequences Asn-X-Ser or Asn-X-Thr (where X is any amino acid except proline) become glycosylated. These two sequences occur much less frequently in glycoproteins than in nonglycosylated cytosolic proteins; evidently there has been selective pressure against these sequences during protein evolution, presumably because glycosylation at too many sites would interfere with protein folding.
is transferred to the asparagine as an
intact unit in a
reaction catalyzed by a membrane-bound oligosaccharyl
transferase enzyme. There is one copy of this
enzyme associated with each protein translocator in the ER membrane.
). The
transfer is catalyzed by a membrane-bound enzyme, an oligosaccharyl
transferase, which has its active site exposed on the luminal side of
the ER membrane; this explains
why cytosolic proteins are not glycosylated in this way. The precursor
oligosaccharide is held in the ER membrane by a special lipid molecule called
dolichol, and it is transferred to the target asparagine in a single
enzymatic step immediately
after that amino acid emerges in the ER lumen during protein translocation
( Figure 12-49). Since most proteins are
co-translationally imported
into the ER, N-linked oligosaccharides are almost always added
during protein
synthesis.
The oligosaccharide is assembled sugar by sugar onto the carrier lipid dolichol (a polyisoprenoid -- see Panel 2-4). Dolichol is long and very hydrophobic: its 22 five-carbon units can span the thickness of a lipid bilayer more than three times, so that the attached oligosaccharide is firmly anchored in the membrane. The first sugar group is linked to dolichol by a pyrophosphate bridge. This high-energy bond activates the oligosaccharide for its transfer from the lipid to an asparagine side chain of a nascent polypeptide on the luminal side of the rough ER. The synthesis of the oligosaccharide starts on the cytosolic side of the ER membrane and continues on the luminal face after the (Man) 5(GlcNAc) 2 lipid intermediate is flipped across the bilayer. All of the subsequent glycosyl transfer reactions on the luminal side of the ER involve transfers from dolichol-P-glucose and dolichol-P-mannose; these activated, lipid-linked monosaccharides are synthesized from dolichol phosphate and UDP-glucose or GDP-mannose (as appropriate) on the cytosolic side of the ER and are then thought to be flipped across the ER membrane. GlcNAc = N-acetylglucosamine; Man = mannose; Glc = glucose.
. The entire oligosaccharide
is built up sugar by sugar on this membrane-bound lipid molecule prior to its
transfer to a protein. The sugars are first activated in the cytosol by the
formation
of nucleotide-sugar intermediates, which then donate their sugar
(directly or
indirectly) to the lipid in an orderly sequence. Partway through this
process, the
lipid-linked oligosaccharide is flipped from the cytosolic to the luminal
side of the
ER membrane ( Figure 12-50).
) and one
mannose residue are quickly removed from the oligosaccharides of most
glycoproteins. This oligosaccharide "trimming" or
"processing" continues in the Golgi
apparatus and is discussed in Chapter 13.
The N-linked oligosaccharides are by far the most common ones found on glycoproteins. Less frequently, oligosaccharides are linked to the hydroxyl group on the side chain of a serine, threonine, or hydroxylysine amino acid. These O-linked oligosaccharides are formed in the Golgi apparatus by pathways that are not yet fully understood (discussed in Chapter 13).
Immediately after the completion of protein synthesis, the precursor protein remains anchored in the ER membrane by a hydrophobic carboxyl-terminal sequence of 15 to 20 amino acids, with the rest of the protein in the ER lumen. Within less than a minute, an enzyme in the ER cuts the protein free from its membrane-bound carboxyl terminus and simultaneously attaches the new carboxyl terminus to an amino group on a preassembled glycosylphosphatidylinositol intermediate. The signal that specifies this modification is contained within the hydrophobic carboxyl-terminal sequence and a few amino acids adjacent to it on the luminal side of the ER membrane; if this signal is added to other proteins, they too become modified in this way. Because of the covalently linked lipid anchor, the protein remains membrane-bound with all of its amino acids exposed initially on the luminal side of the ER and eventually on the cell exterior.
, and it adds a
glycosylphosphatidylinositol (GPI)
anchor, which contains two fatty acids, to the protein. At the same time
the
transmembrane segment of the protein is cleaved off. An increasing number
of plasma
membrane proteins have been shown to be modified in this way. Since these
proteins
are attached to the exterior of the plasma membrane only by their GPI anchors,
in principle they can be released from cells in soluble form in response to
signals that activate a specific phospholipase in the plasma membrane.
Trypanosome parasites, for example, use this mechanism to shed their coat of
GPI-anchored surface proteins if attacked by the immune system.
This phospholipid is synthesized from fatty acyl-coenzyme A (fatty acyl CoA), glycerol 3-phosphate, and cytidine-bisphosphocholine (CDP-choline).
). The two
other major membrane
phospholipidsphosphatidylethanolamine (PE) and phosphatidylserine (PS) - as
well
as the minor phospholipid phosphatidylinositol (PI), are all synthesized in
this way.
Since new lipid molecules are added only to the cytosolic half of the bilayer and lipid molecules do not flip spontaneously from one monolayer to the other, membrane-bound phospholipid translocator proteins ("flippases") are required to transfer selected lipid molecules from the cytosolic half to the luminal half so that the membrane grows as a bilayer. Because the flippase in the ER membrane preferentially recognizes and transfers choline-containing head groups, an asymmetric bilayer is generated, with the luminal monolayer (which produces the outer half of the plasma membrane bilayer) highly enriched for phosphatidylcholine.
).
The ER also produces cholesterol and ceramide. Ceramide is made by condensing the amino acid serine with a fatty acid to form the amino alcohol sphingosine; a second fatty acid is then added to form ceramide. The ceramide is exported to the Golgi apparatus, where it serves as the precursor for the synthesis of two types of lipids: oligosaccharide chains are added to form glycosphingolipids (glycolipids), and phosphocholine head groups are transferred from phosphatidylcholine to other ceramide molecules to form sphingomyelin. Thus both glycolipids and sphingomyelin are produced relatively late in the process of membrane synthesis. Because they are produced by enzymes exposed to the Golgi lumen, they are found exclusively in the noncytosolic half of the lipid bilayers that contain them.
As discussed in Chapter 13, the plasma membrane and the membranes of the Golgi apparatus, lysosomes, and endosomes all form part of a membrane system that communicates with the ER by means of transport vesicles that transfer both proteins and lipids. Mitochondria, plastids, and peroxisomes do not belong to this system, and they require different mechanisms for the import of proteins and lipids for growth. We have already seen that most (for mitochondria and plastids) or all (for peroxisomes) of the proteins in these organelles are imported from the cytosol. Although mitochondria modify some of the lipids they import, they do not synthesize lipids de novo; instead, their lipids have to be imported from the ER, either directly, or indirectly by way of other cellular membranes. In either case, special mechanisms are required for the transfer.
Because phospholipids are insoluble in water, their passage between membranes requires a carrier protein. Phospholipid exchange proteins are water-soluble proteins that carry a single molecule of phospholipid at a time; they can pick up a lipid molecule from one membrane and release it at another and thereby redistribute phospholipids between membrane-bounded compartments. The transfer of phosphatidylcholine (PC) from ER to mitochondria can occur without the input of additional energy because the concentration of PC is high in the ER membrane (where it is made) and low in the mitochondrial outer membrane. One would predict that there must be a flippase in the outer mitochondrial membrane to equilibrate the lipids between the two leaflets of the bilayer, and there must be a mechanism to transfer lipids between the outer and inner mitochondrial membrane. These postulated pathways, however, remain to be discovered.
). It
has been proposed that phosphatidylserine is imported into mitochondria in
this
way and then decarboxylated to yield phosphatidylethanolamine, while
phosphatidylcholine is imported intact.
Exchange proteins act to distribute phospholipids at random among all membranes present. In principle, such a random exchange process can result in a net transport of lipids from a lipid-rich to a lipid-poor membrane, allowing phosphatidylcholine and phosphatidylserine molecules, for example, to be transferred from the ER, where they are synthesized, to a mitochondrial or peroxisomal membrane. It might be that mitochondria and peroxisomes are the only "lipid-poor" organelles in the cytosol and that such an exchange process is sufficient, although other, more specific mechanisms probably also exist for transporting phospholipids to these organelles.
The extensive ER network serves as a factory for the production of almost all of the cell's lipids. In addition, a major portion of the cell's protein synthesis occurs on the cytosolic surface of the ER: all proteins destined for secretion and all proteins destined for the ER itself, the Golgi apparatus, the lysosomes, the endosomes, and the plasma membrane are first imported into the ER from the cytosol. In the ER lumen, the proteins fold and oligomerize, disulfide bonds are formed, and N-linked oligosaccharides are added.
Only proteins that carry a special hydrophobic signal peptide are imported into the ER. The ER signal peptide is recognized by a signal recognition particle (SRP), which binds both the growing polypeptide chain and the ribosome and directs them to a receptor protein on the cytosolic surface of the rough ER membrane. This binding to the membrane initiates the translocation process that threads a loop of polypeptide chain across the ER membrane through a hydrophilic pore in a protein translocator.
Soluble proteins destined for the ER lumen, for secretion, or for transfer to the lumen of other organelles pass completely into the ER lumen. Transmembrane proteins destined for the ER or for other cell membranes are translocated across the ER membrane but are not released into the lumen; instead, they remain anchored in the lipid bilayer by one or more membrane-spanning alpha-helical regions in their polypeptide chain. These hydrophobic portions of the protein can act either as start-transfer or stop-transfer signals during the translocation process. When a polypeptide contains multiple alternating start-transfer and stop-transfer signals, it will pass back and forth across the bilayer multiple times.
The asymmetry of lipid synthesis, protein insertion, and glycosylation in the ER establishes the polarity of the membranes of all of the other organelles that the ER supplies with lipids and membrane proteins.
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