Requirement of the TCR ζ chain for binding of NAK/p62 to Nef. (A) In vitro kinase assay after immunoprecipitation (IP) of CD8-Nef chimeras using the CD8 tag from stably transfected wild-type and mutant Jurkat cell lines lacking Lck, TCR, or CD45. Lane 1, control (Cont.) Jurkat transfected with the CD8 tag. (B) Control immunoprecipitation showing expression of ³⁵S-labeled CD8-Nef. (C) In vitro kinase assay after immunoprecipitation of CD8-Nef to study NAK/p62 association/phosphorylation in wild-type (Cont., lane 1) and TCR⁻ Jurkat cell lines (lane 2), and after coexpression (stable transfection) of CD8-Nef with either CD16ε, CD16ζ2 (ITAM 2), CD16ζ3 (ITAM 3), or CD16ζmu (mutation of all three ITAMs) in the TCR⁻ cell line (lanes 3–6). (D) Control immunoprecipitation of ³⁵S-labeled CD8-Nef from cell lines shown in C. (E) In vitro kinase assay after immunoprecipitation of AU-1–tagged Nef from transiently transfected 293T cells. Lane 1, transfection with Nef alone; lanes 2–7, cotransfection with increasing amounts (0.5 and 1 μg) of CD16ε, CD16ζ, or CD16ζmu. (F) The nitrocellulose filter shown in E was blotted (WB) with an anti-Nef (AU-1) antibody to verify comparable Nef expression.

Association of membrane-associated Nef with the TCR ζ chain. (A) Anti-Nef (CD8) immunoprecipitation, then anti-ζ Western blot (WB). (B) Anti-ζ immunoprecipitation, then anti-Nef Western blot from wild-type Jurkat cells stably transfected with CD8 tag (Cont.), and CD8-Nef chimeras containing full-length Nef expressed in the cytoplasm (CD8.Nef.cyt.), the NH₂-terminal 49 amino acids of Nef (CD8-Nef.49), the NH₂-terminal 94 amino acids (CD8-Nef.94), and CD8-Nef.94PXmu in which the PxxP motif has been mutated. (C) Control immunoprecipitation of CD8.Nef chimeras from ³⁵S-labeled cells to show a comparable protein expression (*). (D) Nef–ζ association after baculovirus coinfection of Hi5 cells. Control anti-Nef Western blot (WB) after anti-Nef (AU-1) immunoprecipitation from Hi5 cells infected with wild-type Nef or Nef with a mutated PxxP motif (lanes 1 and 2). Immunoprecipitated Nef from Hi5 cells ran, in addition to monomers (Nef-m), as dimers (Nef-d) or higher order multimers (arrows), which may be important for Nef function. Hi5 cells were then coinfected with wild-type Nef and ζ fused to CD16 (CD16ζ; lanes 3–6). CD16ζ was immunoprecipitated using an AU-5 tag, and the immunoprecipitates were blotted for Nef (AU-1). Two immunoprecipitations were performed in the presence of cytoplasmic lysates from Jurkat (ζ-positive; lane 4) or TCR-ζ–negative cells (lane 5). The positions of the antibody heavy (*) and light (**) chains are indicated. (E) Control Western blot. The nitrocellulose filter shown in D was stripped and blotted with an antibody recognizing the CD16ζ construct (AU-5).

Nef is required for FasL upregulation. Jurkat cells were infected with (A) wild-type HIV-1 (NL4-3.SF2Nef) or (B) SF2 lacking the nef gene (NL4-3ΔNef). After 48 h, FasL expression (solid line) was assessed by flow cytometry and compared with staining with a control mAb (dashed line). The level of viral replication in Jurkat cells was comparable as determined by RT activity (NL4-3.SF2Nef, 4.6 × 10³ cpm; NL4-3ΔNef, 5.8 × 10³ cpm).

FasL upregulation by HIV requires the TCR ζ chain. FasL expression was assessed 48 h after infection with HIV (IIIB strain) by immunoprecipitation using an anti-FasL mAb (A) or by flow cytometry (B). Wild-type (WT) and TCR⁻ Jurkat are compared with the TCR⁻ cells stably transfected with CD16ζ or CD16ζmu (signaling-defective CD16ζ). The level of viral replication in Jurkat cells was comparable as determined by p24 assay (wild-type, 3.5 ± 0.5; TCR⁻, 3.8 ± 1.0; CD16ζ, 3.8 ± 0.5; CD16ζmu, 3.1 ± 0.25 ng/ml).

Induction of FasL expression by Nef or a Nef mutant (Nef.PXmu). Jurkat cells were transfected with CD8-Nef or CD8-Nef.PXmu (no binding to TCR-ζ) construct by electroporation and kept under neomycin selection for 2 wk. Outgrowing cells were selected for CD8 surface expression by Dynabeads and analyzed for FasL expression by FACS^® as described above.

Upregulation of FasL by Nef requires TCR-ζ. Transient cotransfection of a FasL promotor/luciferase reporter with an empty vector (cont.; negative control), Tax (positive control), Nef, and Nef.PXmu into Jurkat (WT), TCR⁻ Jurkat (TCR⁻), and TCR⁻ cells reconstituted with CD16-ζ (TCR⁻/Zeta). The expression of the reporter gene was determined as described in Materials and Methods. Bars, the mean ± SD of three experiments.

Model describing mechanisms of immune evasion mediated by the HIV nef gene. Nef is expressed in the early viral life cycle and, after myristoylation, associates with the plasma membrane where several protein interactions take place. Nef interacts with ζ, which leads to the activation of p62/ NAK, which in turn causes the binding of p62/NAK to Nef. These events ultimately stimulate FasL expression, which may protect infected cells from CTL attack by killing Fas⁺ viral-specific CTLs in the process (1). Nef can also downregulate MHC class I expression and protect the infected cells against killing by CTLs (2), or CD4 expression leading to loss of CD4 T cell function (2).