CD44 is a ubiquitous multistructural and multifunctional cell surface adhesion molecule involved in cell-cell and cell-matrix interactions. It is the most studied alternatively spliced gene in cancer. Of its 20 exons, the first and last five exons are constant, whereas the 10 intermediate exons are subject to alternative splicing, resulting in the generation of a variable region. Differential utilization of the 10 variable region exons generates multiple isoforms of different molecular sizes (85 to 230 kDa), as do variations in N-glycosylation, O-glycosylation, and glycosaminoglycanation. This fact implicates CD44 in a variety of responses, including lymphocyte homing, hematopoiesis, inflammation, tumorigenesis, angiogenesis, and metastasis. The smallest CD44 molecule (85 to 95 kDa), which lacks the entire variable region, is the standard form (CD44s). CD44s is a single-chain molecule composed of a distal extracellular domain (containing the ligand-binding sites), a membrane-proximal region, a transmembrane-spanning domain, and a cytoplasmic tail. A CD44 isoform containing the last three exon products of the variable region, CD44V8–10 (also known as epithelial CD44 or CD44E), is preferentially expressed on epithelial cells. Whereas the CD44s is widely expressed and HA is ubiquitous in most extracellular spaces, variant isoforms of CD44 have restricted expression to specific conditions, such as transformation, wound healing, and lymphocyte activation.⁶

In theory, CD44 has the basic structure necessary to function in signal transduction. However, the CD44 cytoplasmic tail exhibits no inherent receptor kinase or phosphatase activity. ECM outside-in CD44 signaling is communicated through various mechanisms: 1) direct CD44 signaling, for which HA binding initiates extracellular clustering of CD44, resulting in the activation of kinases, such as c-Src and FAK as well as Rho and Rac^7,8,9; this activation leads to enhanced association of CD44 into actin cytoskeleton complexes as well as recruitment and activation of additional signaling partners that potentiate cell migration¹⁰; 2) CD44 serving as a co-receptor physically linked to other classical signaling receptors, such as c-Met,¹¹ members of the ErbB family of receptor tyrosine kinases,^12,13 and transforming growth factor-βR1,^14,15,16 and in the process, facilitating the association of intracellular mediators of signal transduction; 3) CD44 functioning as a docking protein for pericellular proteins, such as matrix metalloproteinases,^17,18 or for cytoplasmic proteins, such as kinases, Smad1, actin-binding proteins, and other adapter proteins that can subsequently activate signaling pathways; 4) direct CD44-mediated signaling occurring as a two-step process: γ-secretase cleavage of the transmembrane domain and the subsequent release of CD44 intracellular domain, which exhibits nuclear translocation and functions as a transcription factor of target genes, such as CD44 itself.¹⁹

Recently, we have generated a Tet Off-regulated CD44 expression in a weakly metastatic breast cancer cell line exhibiting low endogenous expression of CD44 and have demonstrated that induction of CD44s increased the migration and invasiveness of MCF7F-B5 cells through an experimental matrix.²⁶ To test this in vitro observation and determine the precise role of CD44s in tumor growth and metastasis, we developed an in vivo Tet Off-regulated CD44 expression system, using a breast cancer xenograft mouse model. Comparing these mice to control mice, we showed that: induction of CD44s resulted in metastasis of MCF7F-B5-primary breast tumors to the liver but did not affect either the formation or growth rate of the primary tumor, and both primary and secondary tumors expressed high levels of CD44. These data confirmed our previous in vitro results,²⁶ clearly demonstrating that up-regulation of CD44s can promote breast tumor metastasis to the liver. To understand better the molecular mechanisms implicated in CD44s downstream signaling-mediated breast tumor invasion, we used gene profiling technology, which allowed us to identify a number of potential CD44s downstream transcriptional targets,²⁶ and experiments aiming to validate their functional role in CD44s-promoted breast cell invasion and metastasis are underway.

Several researchers have concluded that CD44s promotes tumor progression and metastasis, whereas others maintain that CD44s inhibits this process. Using MMTV-PyV mT mice crossed onto a CD44^−/− background, Lopez and colleagues³⁰ reported the absence of CD44-induced breast cancer metastasis to the lung, suggesting that HA binding to an alternate receptor, such as RHAMM or LYVE-1, may attenuate breast cancer cell invasion. It has to be emphasized that, although breast cancer cell lines can express both standard and variant isoforms, the CD44^−/− mouse model cells are lacking all forms of CD44.³⁰ Compared to the MMTV-PyV mT/CD44^−/− mouse model,³⁰ the advantage of the Tet Off-regulated CD44 expression breast cancer xenograft mouse model described in the present study is that the effect of a selected human CD44, CD44s, can be evaluated. Several studies have provided strong evidence to support our findings that CD44s can facilitate breast tumor cell invasion and metastasis.^{30,31,32,33,34} The hypothesis that CD44 plays a potential role in metastasis originated from the simple observation that the CD44v6 variant conferred metastatic ability to a previously nonmetastatic rat pancreatic carcinoma cell line.³¹ Conversely, antisense CD44 transfection has been shown to inhibit tumor growth and metastasis in highly metastatic mammary carcinoma cells.³⁵ Human breast carcinoma samples examined by different techniques were found to contain primarily CD44E isoform in the normal breast tissue whereas metastatic breast carcinomas appeared to overexpress CD44s and variant isoforms.⁵

Previous studies using IHC have reported a wide range of anti-CD44s positivity in invasive breast carcinoma, from 26 to 62%.^36,37,38,39 The expression of CD44s and CD44v6 was associated with the invasion and metastasis of breast carcinoma.⁴⁰ CD44-HA interaction seemed to be cell-type-specific and dependent on CD44 isoform expression during cancer progression and metastatic spread. Also, HA has been shown to promote breast cancer cell invasion in vitro through activation of CD44.⁴¹ Additional studies have also identified a number of partners that CD44 may interact with to promote cell signaling that mediates tumor progression. Examples include c-Src, ErbB2, ankyrin, and the ERM proteins.^7,12,42 Whereas HA is highly expressed and even induced in the ECM of these tumors, induction of its primary receptor in weakly invasive MCF7F-B5 breast cancer cell line resulted in an increase in tumor metastasis to the liver. This finding implicates CD44s/HA interaction in breast tumor invasion. Previous studies have established a positive correlation between cell invasiveness and increased expression of HAS2 (HA synthase 2), HA, HYAL2 (hyaluronidase 2), and CD44.⁴³ Udabage and colleagues⁴³ have recently shown that antisense inhibition of HAS2 resulted in accumulation of high molecular weight HA and a decrease in CD44 and HYAL2, resulting in attenuated cellular proliferation and in vitro invasiveness, and inhibited the formation of primary and secondary tumors in vivo.⁴⁴ Expression levels of HAS2, HA, and HYAL2 will be examined in the same samples obtained in the present study. These data support our finding that CD44s might play an important role, not only in the initiation of secondary tumors but also in their growth. Furthermore, our previous in vitro model strongly supports the present data.²⁶ Induction of CD44 expression on the weakly motile MCF7F-B5 cells increased the migratory and invasive properties of this breast cancer cell line in HA-supplemented Matrigel. In addition, depletion of CD44 expression on the breast cancer cell lines MDA-MB-231 and MDA-MB-157 cells both reduced the invasiveness of these cells and decreased the adhesion of these cells to human bone marrow endothelial cells.⁴⁵ Conversely, the adhesion of each of the CD44-negative breast cancer and prostate cancer cell lines (T47D, MCF-7, and DU145) to human bone marrow endothelial cells was dramatically increased after transfection of these cells to express CD44s.⁴⁵

Studies using MCF-7 breast xenograft models have observed metastasis to the liver and other organs such as bone and lung.^46,47 In the present study, metastasis of the primary breast tumor cells MCF7F-B5 was seen in the liver only. This observation might be explained by the activation of specific pathway(s) on induction of CD44s in the MCF7-B5 cells leading to a liver-specific metastasis. Breast cancer cells with CD44⁺/CD24⁻ subpopulation have been shown to express higher levels of proinvasive genes and have highly invasive properties,²¹ supporting cortactin as a newly identified target for CD44-promoted breast tumor invasion/metastasis.²⁶ Ongoing validation experiments in our laboratory are aiming to further identify potential CD44s downstream target genes that might play a key role in the organotropism of breast cancer metastasis.⁴⁸ Although metastasis to the liver is observed infrequently in patients with breast cancer at initial presentation, it portends a worse clinical outcome.⁴⁹ Metastatic breast cancer to the liver contributes to a shorter median survival rate, reported to be in the range of 3 to 14 months.⁵⁰ Although the liver is the site of metastasis in 5 to 20% of women with metastatic breast cancer,⁵⁰ liver metastasis rarely occurs in women with ductal carcinoma in situ. Our data indicate that CD44s might be involved in facilitating aggressive dissemination of breast cancer tumors to the liver.