2008
DOI: 10.1099/vir.0.83226-0
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Functional analysis of human cytomegalovirus pUS28 mutants in infected cells

Abstract: The human cytomegalovirus (HCMV)-encoded viral G protein-coupled receptor pUS28 contributes to an array of biological effects, including cell migration and proliferation. Using FIX-BAC (bacterial artificial chromosome, derived from the HCMV clinical isolate VR1814) and lambda red recombination techniques, we generated HCMV recombinants expressing amino-terminally FLAG-tagged versions of wild-type pUS28 (FLAG–US28/WT), G-protein coupling deficient pUS28 (FLAG–US28/R129A) and chemokine-binding domain deficient p… Show more

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Cited by 28 publications
(36 citation statements)
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“…Bacterial artificial chromosomes (BACs) containing either the wild-type VR1814 strain of HCMV (FIX-BAC) or a mutant in which the US28 open reading frame was replaced by a Kan r /LacZ cassette (FIX-BAC-⌬US28) have been previously described (16,49). Lambda red recombination was utilized to construct a mutant of US28 termed US28/1-314 from which amino acids 315 to 354 have been deleted.…”
Section: Methodsmentioning
confidence: 99%
“…Bacterial artificial chromosomes (BACs) containing either the wild-type VR1814 strain of HCMV (FIX-BAC) or a mutant in which the US28 open reading frame was replaced by a Kan r /LacZ cassette (FIX-BAC-⌬US28) have been previously described (16,49). Lambda red recombination was utilized to construct a mutant of US28 termed US28/1-314 from which amino acids 315 to 354 have been deleted.…”
Section: Methodsmentioning
confidence: 99%
“…35kDa). Although counter-intuitive, this result is consistent with published data suggesting that the deleted region of the N-terminus may be a site of post-translational modification, possibly O-linked glycosylation Stropes & Miller, 2008). Data from B105 sequencing confirmed the correct sequence, whereas B182 lacked the deletion.…”
Section: Bac Recombinneringsupporting
confidence: 81%
“…For example, M33 of mouse CMV has a variant NRY motif at this position; N-D mutation resulted in enhanced signalling, whereas R-Q resulted in ablation of signalling (Case et al, 2008). Similarly, an R-A mutation on US28 resulted in a signalling deficient phenotype (Stropes & Miller, 2008). Here, the D128N substitution, which retained >70% of CREB activation levels compared with wt UL33, did not affect migration in contrast to the signalling deficient R129Q mutation.…”
Section: Discussionmentioning
confidence: 76%
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