Entropic switch regulates myristate exposure in the HIV-1 matrix protein

Tang, Chun; Loeliger, Erin; Luncsford, Paz J.; Kinde, Isaac; Beckett, Dorothy; Summers, Michael F.

doi:10.1073/pnas.0305665101

Cited by 296 publications

(541 citation statements)

References 66 publications

(52 reference statements)

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“…One would therefore predict that addition of the CA domain, which contains additional multimerization signals, should promote myristate exposure at lower protein concentrations than myrMA. This is exactly what Tang et al (11) found. The monomer 7 trimer equilibrium constant is 20 times higher for myrMA-CA than for myrMA.…”

supporting

confidence: 77%

A myristoyl switch regulates membrane binding of HIV-1 Gag

Resh

2004

Proc. Natl. Acad. Sci. U.S.A.

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supporting

confidence: 77%

A myristoyl switch regulates membrane binding of HIV-1 Gag

Resh

2004

Proc. Natl. Acad. Sci. U.S.A.

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“…NOEs between the myristate group and the side chains of Val-7 and Leu-8 were also observed for the WT myrMA protein. 27 These NMR observations indicate that mutation of Arg-7 and Leu-8 does not greatly alter the conformation of the loop and that residues 7 and 8 play an important role into the stabilization of the myr(s) form.…”

Section: Nmr Analysis Of V7r- L8a-and L8i-myrmamentioning

confidence: 77%

“…In addition, the relative NOE intensities and cross-peak patterns matched the data obtained for the WT myr(s)MA protein. 27,31 The main differences between the structures are localized within the disordered loop formed by residues Gly-2 -Ser-9. For V7R, the side chain of Arg-7 is poised to make a salt bridge with the side chain of Glu-52, and the mythelene groups of Arg-7 contribute to the hydrophobic interactions with the methylene groups of the myristate ( Figure 6).…”

Section: Structures Of V7r-and L8a-myrmamentioning

confidence: 99%

“…In contrast, for the wild type (WT) myrMA protein, a subset of signals shift progressively toward the frequencies observed for myr(-)MA upon increasing the protein concentration due to a concomitant shift in the monomer-trimer equilibrium toward the trimeric species and exposure of the myristyl group. 27 The absence of concentration-dependent shifts for V7R, L8A, and L8I indicates that these mutants exist in a unique conformation over the range of concentrations tested. Sedimentation equilibrium (SE) data obtained for V7R, L8A and L8I are similar in appearance to SE data obtained for myr(-) MA, and confirm that the myrMA mutants remain monomeric at concentrations as high as 1 mM.…”

Section: Introductionmentioning

confidence: 98%

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Point Mutations in the HIV-1 Matrix Protein Turn Off the Myristyl Switch

Saad¹,

Loeliger²,

Luncsford³

et al. 2007

Journal of Molecular Biology

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102

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During the late phase of HIV-1 replication, newly synthesized retroviral Gag proteins are targeted to lipid raft regions of specific cellular membranes, where they assemble and bud to form new virus particles. Gag binds preferentially to the plasma membrane (PM) of most hematopoietic cell types, a process mediated by interactions between the cellular PM marker phosphatidylinositol-(4,5)-bisphosphate (PI(4,5)P 2 ) and Gag's N-terminally-myristoylated matrix (MA) domain. We recently demonstrated that PI(4,5)P 2 binds to a conserved cleft on MA and promotes myristate exposure, suggesting a role as both a direct membrane anchor and myristyl switch trigger. Here we show that PI(4,5)P 2 is also capable of binding to MA proteins containing point mutations that inhibit membrane binding in vitro, and in vivo, including V7R, L8A and L8I. However, these mutants do not exhibit PI(4,5)P 2 -or concentration-dependent myristate exposure. NMR studies of V7R and L8A MA reveal minor structural changes that appear to be responsible for stabilizing the myristate-sequestered (myr (s)) species and inhibiting exposure. Unexpectedly, the myristyl group of a revertant mutant with normal PM targeting properties (V7R,L21K) is also tightly sequestered and insensitive to PI(4,5) P 2 binding. This mutant binds PI(4,5)P 2 with two-fold higher affinity compared with the native protein, suggesting a potential compensatory mechanism for membrane binding. KeywordsHuman immunodeficiency virus type-1 (HIV-1); Gag; myristyl (myr); matrix (MA); phosphatidylinositol-4,5-bisphosphate (PI(4,5)P 2 ); analytical ultracentrifugation (AU); nuclear magnetic resonance (NMR)

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“…A decade ago, it was proposed that the interaction of the MA domain of Pr55 Gag with membrane is regulated by a myristyl switch (12), and a substantial amount of evidence supports this model (13)(14)(15). Most recently, structural studies from Summers and colleagues (16) demonstrated that the myristate is sequestered when MA is in a monomeric form, which binds membrane poorly. In contrast, when downstream sequences in CA that promote oligomerization are added to MA, the myristate becomes exposed, and membrane binding is substantially increased.…”

mentioning

confidence: 99%

HIV-1 Gag: Flipped out for PI(4,5)P ₂

Freed

2006

Proc. Natl. Acad. Sci. U.S.A.

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Entropic switch regulates myristate exposure in the HIV-1 matrix protein

Cited by 296 publications

References 66 publications

A myristoyl switch regulates membrane binding of HIV-1 Gag

A myristoyl switch regulates membrane binding of HIV-1 Gag

Point Mutations in the HIV-1 Matrix Protein Turn Off the Myristyl Switch

HIV-1 Gag: Flipped out for PI(4,5)P ₂

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Entropic switch regulates myristate exposure in the HIV-1 matrix protein

Cited by 296 publications

References 66 publications

A myristoyl switch regulates membrane binding of HIV-1 Gag

A myristoyl switch regulates membrane binding of HIV-1 Gag

Point Mutations in the HIV-1 Matrix Protein Turn Off the Myristyl Switch

HIV-1 Gag: Flipped out for PI(4,5)P 2

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HIV-1 Gag: Flipped out for PI(4,5)P ₂