Amino acid substitutions within the matrix protein of type D retroviruses affect assembly, transport and membrane association of a capsid.

Rhee, Sehun; Hunter, Eric

doi:10.1002/j.1460-2075.1991.tb07980.x

Cited by 89 publications

(110 citation statements)

References 43 publications

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“…Following separation of proteins by SDS-PAGE, the band intensity of Pr78 was measured for wild type and each mutant using phosphorimaging. Eighty percent of pulse-labeled Gag polyprotein was incorporated into immature capsids for wild type and A18V, a mutant that accumulates capsids in the cytoplasm (25). R55W, a mutant that assembles capsids at the plasma membrane (27), demonstrated only 50% Gag polyprotein was incorporated into capsids after the 30-min chase.…”

Section: Construction Of M-pmv Matrix Mutantsmentioning

confidence: 99%

“…To better define the kinetics with which mutant Gag proteins were released and processed, a pulse-chase experiment with multiple chase times (1, 2, and 4 h) was carried out. This laboratory has previously shown that Gag precursor processing and virus release are temporally linked and that in the absence of capsid release Gag processing is not observed (25). Following analysis of samples with SDS-PAGE, OptiQuant software was used to obtain the band intensities for Gag (Pr78), Gag-Pro (p95), Gag-Pro-Pol (p180), and capsid (p27).…”

Section: Construction Of M-pmv Matrix Mutantsmentioning

confidence: 99%

“…This means that instead of simultaneously extruding the membrane as they assemble, assembled betaretrovirus capsids must interact with the plasma membrane in a way that stimulates wrapping of the spherical structure with the lipid bilayer. The matrix (MA) domain of the M-PMV Gag polyprotein plays a critical role in this process (25), as well as in directing translating polysomes to the intracellular assembly site (32) and subsequent transport to the plasma membrane (8,25,27,32). MA is cotranslationally modified with myristic acid, a 14-carbon saturated fatty acid, and while myristylation of this domain is dispensable for capsid assembly, it is required for transport and release of capsids (26,29).…”

mentioning

confidence: 99%

“…Based on a nuclear magnetic resonance (NMR) analysis of the M-PMV matrix protein, which is comprised of four helical domains arranged in two perpendicularly aligned pairs (9), and on an MA mutant (T41I/T78I) that accumulated immature capsids at the plasma membrane (25), it was previously hypothesized that the myristic acid moiety is sequestered within the MA domain prior to plasma membrane interactions (9). T41I/ T78I immature capsids are assembled and transported to the plasma membrane with wild-type kinetics but are defective at an early stage of budding (25).…”

mentioning

confidence: 99%

“…T41I/ T78I immature capsids are assembled and transported to the plasma membrane with wild-type kinetics but are defective at an early stage of budding (25). Because the structural analyses showed that both of the threonine residues replaced in this mutant are oriented toward the core of the matrix protein, it was reasoned that substitution with the hydrophobic isoleucine residues might prevent release of myristic acid from the more hydrophobic MA core, even after the T41I/T78I capsid interacted with the lipid bilayer (9).…”

mentioning

confidence: 99%

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An Early Stage of Mason-Pfizer Monkey Virus Budding Is Regulated by the Hydrophobicity of the Gag Matrix Domain Core

Stansell

Tytler

Walter

et al. 2004

J Virol

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Intracellular capsid transport and release of Mason-Pfizer monkey virus are dependent on myristylation of the Gag matrix domain (MA). A myristylated MA mutant, in which Thr41 and Thr78 are replaced with isoleucines, assembles capsids that are transported to the plasma membrane but are blocked in an early budding step. Since the nuclear magnetic resonance structure of MA showed that these Thr residues point into the hydrophobic core of the protein, it was hypothesized that the T41I/T78I mutant was defective in release of myristic acid from the more hydrophobic core. In order to further investigate whether an increase in the hydrophobicity of the MA core modulates capsid-membrane interactions and viral budding, three tyrosine residues (11, 28, and 67), oriented toward the MA core, were replaced individually or in a pair-wise combination with the more hydrophobic phenylalanine residue(s). As a control, Tyr82, oriented toward the outer surface of MA, was also replaced with phenylalanine. These Tyr-to-Phe substitutions did not alter capsid assembly compared to wild type in a capsid assembly assay. Pulse-chase, immunofluorescence, and electron microscopy studies demonstrated that single substitutions of Tyr11, Tyr28, and Tyr67 recapitulated the T41I/T78I mutant phenotype of decreased budding kinetics and accumulation of capsids at the plasma membrane. MA double mutants with a combination of these Tyr substitutions exhibited a phenotype that was even more defective in budding. In contrast, MA mutants with Tyr82 replaced by Phe resulted in a transportdefective phenotype. These results strongly support the hypothesis that myristic acid is sequestered inside MA prior to capsid-membrane interactions.

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Section: Construction Of M-pmv Matrix Mutantsmentioning

confidence: 99%

Section: Construction Of M-pmv Matrix Mutantsmentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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An Early Stage of Mason-Pfizer Monkey Virus Budding Is Regulated by the Hydrophobicity of the Gag Matrix Domain Core

Stansell

Tytler

Walter

et al. 2004

J Virol

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Molecular aspects of the interaction between Mason—Pfizer monkey virus matrix protein and artificial phospholipid membrane

et al. 2016

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The Mason-Pfizer monkey virus is a type D retrovirus, which assembles its immature particles in the cytoplasm prior to their transport to the host cell membrane. The association with the membrane is mediated by the N-terminally myristoylated matrix protein. To reveal the role of particular residues which are involved in the capsid-membrane interaction, covalent labelling of arginine, lysine and tyrosine residues of the Mason-Pfizer monkey virus matrix protein bound to artificial liposomes containing 95% of phosphatidylcholine and 5% phosphatidylinositol-(4,5)-bisphosphate (PI(4,5)P ) was performed. The experimental results were interpreted by multiscale molecular dynamics simulations. The application of these two complementary approaches helped us to reveal that matrix protein specifically recognizes the PI(4,5)P molecule by the residues K20, K25, K27, K74, and Y28, while the residues K92 and K93 stabilizes the matrix protein orientation on the membrane by the interaction with another PI(4,5)P molecule. Residues K33, K39, K54, Y66, Y67, and K87 appear to be involved in the matrix protein oligomerization. All arginine residues remained accessible during the interaction with liposomes which indicates that they neither contribute to the interaction with membrane nor are involved in protein oligomerization. Proteins 2016; 84:1717-1727. © 2016 Wiley Periodicals, Inc.

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Three-Dimensional Structure of the HTLV-II Matrix Protein and Comparative Analysis of Matrix Proteins from the Different Classes of Pathogenic Human Retroviruses

Christensen

Massiah

Turner

et al. 1996

Journal of Molecular Biology

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Amino acid substitutions within the matrix protein of type D retroviruses affect assembly, transport and membrane association of a capsid.

Cited by 89 publications

References 43 publications

An Early Stage of Mason-Pfizer Monkey Virus Budding Is Regulated by the Hydrophobicity of the Gag Matrix Domain Core

An Early Stage of Mason-Pfizer Monkey Virus Budding Is Regulated by the Hydrophobicity of the Gag Matrix Domain Core

Molecular aspects of the interaction between Mason—Pfizer monkey virus matrix protein and artificial phospholipid membrane

Three-Dimensional Structure of the HTLV-II Matrix Protein and Comparative Analysis of Matrix Proteins from the Different Classes of Pathogenic Human Retroviruses

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