Vif determines the requirement for CBF-β in APOBEC3 degradation

Yoshikawa, Rokusuke; Takeuchi, Junko; Yamada, Eri; Nakano, Yoshiaki; Ren, Fengrong; Tanaka, Hiroshi; Münk, Carsten; Harris, Reuben S.; Miyazawa, Takayuki; Koyanagi, Yoshio; Sato, Kei

doi:10.1099/jgv.0.000027

Cited by 16 publications

(22 citation statements)

References 41 publications

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“…However, some cross degradation was observed as might also be expected because the A3 enzymes are relatively conserved (especially in comparison to Vif). Surprisingly, recent work has demonstrated that CBF-β is specifically required for function of primate lentiviral Vif proteins, but not for non-primate Vifs (Ai et al, 2014; Han et al, 2014; Yoshikawa et al, 2014; Zhang et al, 2014). These data indicate that either the Vif proteins of FIV, BIV, and MVV do not require a CBF-β-like factor, or these viruses have evolved to use one or more other as-yet-unknown cellular factors.…”

Section: Human Apobec3 Enzymes and Hiv Restrictionmentioning

confidence: 99%

APOBECs and virus restriction

2015

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The APOBEC family of single-stranded DNA cytosine deaminases comprises a formidable arm of the vertebrate innate immune system. Pre-vertebrates express a single APOBEC, whereas some mammals produce as many as eleven enzymes. The APOBEC3 subfamily displays both copy number variation and polymorphisms, consistent with ongoing pathogenic pressures. These enzymes restrict the replication of many DNA-based parasites, such as exogenous viruses and endogenous transposable elements. APOBEC1 and activation-induced cytosine deaminase (AID) have specialized functions in RNA editing and antibody gene diversification, respectively, whereas APOBEC2 and APOBEC4 appear to have different functions. Nevertheless, the APOBEC family protects against both periodic viral zoonoses as well as exogenous and endogenous parasite replication. This review highlights viral pathogens that are restricted by APOBEC enzymes, but manage to escape through unique mechanisms. The sensitivity of viruses that lack counterdefense measures highlights the need to develop APOBEC-enabling small molecules as a new class of anti-viral drugs.

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Section: Human Apobec3 Enzymes and Hiv Restrictionmentioning

confidence: 99%

APOBECs and virus restriction

2015

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“…This cross-species “jump” was most likely facilitated by hijacking CBF-β to counteract APOBEC3-mediated restriction through the aforementioned two-pronged mechanism (Fig 1D). In support of this model, SIV Vif still has the capacity to degrade feline APOBEC3 enzymes in a CBF-β dependent manner [10, 24, 25]. Moreover, this newly transmitted virus most likely initially produced a Vif protein capable of suboptimal degradation of the APOBEC3 enzymes of its new host.…”

Section: Introductionmentioning

confidence: 99%

Evolutionary Paradigms from Ancient and Ongoing Conflicts between the Lentiviral Vif Protein and Mammalian APOBEC3 Enzymes

Harris

Anderson

2016

PLoS Pathog

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“…Next, we used an in vitro cell culture system to evaluate whether FIVpco Vif can degrade feline APOBEC3 proteins. For this assay, we obtained the FLAG‐tagged codon‐optimized open reading frames of FIVfca Vif strain Petaluma , FIVfca strain C36 and FIVpco strain PLV1695 from GeneArt Gene Synthesis service (Life Technologies, Carlsbad, CA, USA) (the GenBank accession numbers are presented in the legend of Figure , and the codon‐optimized sequences are available on request). The obtained DNA fragments were inserted the Bam HI‐ Sal I site of pDON‐AI plasmid (Takara, Kyoto, Japan).…”

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“…We co‐transfected these plasmids into HEK293T cells by using PEI Max (Polysciences, Warrington, PA, USA) and harvested the cells and viral particles from culture supernatants at 48 hr post‐transfection. The harvested samples were used for SDS‐PAGE/western blotting or lentiviral reporter assays as previously described . Briefly, we used the following antibodies for western blotting: an anti‐FLAG polyclonal antibody (Sigma, St Louis, MO, USA), an anti‐HA antibody (3F10; Roche, Indianapolis, IN, USA), an anti‐FIV p27 Capsid antibody (PAK3‐2C1; Santa Cruz Biotechnology, Santa Cruz, CA, USA); an anti‐α‐tubulin antibody (DM1A; Sigma) and an anti‐VSVg antibody (P5DA; Roche).…”

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Species‐specific differences in the ability of feline lentiviral Vif to degrade feline APOBEC3 proteins

Yoshikawa

Nakano

Yamada

et al. 2016

Microbiology and Immunology

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How host–virus co‐evolutionary relationships manifest is one of the most intriguing issues in virology. To address this topic, the mammal–lentivirus relationship can be considered as an interplay of cellular and viral proteins, particularly apolipoprotein B mRNA editing enzyme catalytic polypeptide‐like 3 (APOBEC3) and viral infectivity factor (Vif). APOBEC3s enzymatically restrict lentivirus replication, whereas Vif antagonizes the host anti‐viral action mediated by APOBEC3. In this study, the focus was on the interplay between feline APOBEC3 proteins and two feline immunodeficiency viruses in cats and pumas. To our knowledge, this study provides the first evidence of non‐primate lentiviral Vif being incapable of counteracting a natural host's anti‐viral activity mediated via APOBEC3 protein.

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Vif determines the requirement for CBF-β in APOBEC3 degradation

Cited by 16 publications

References 41 publications

APOBECs and virus restriction

APOBECs and virus restriction

Evolutionary Paradigms from Ancient and Ongoing Conflicts between the Lentiviral Vif Protein and Mammalian APOBEC3 Enzymes

Species‐specific differences in the ability of feline lentiviral Vif to degrade feline APOBEC3 proteins

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