Mutations in human cytomegalovirus UL97 gene confer clinical resistance to ganciclovir and can be detected directly in patient plasma.

Wolf, Dana; Smith, Irene L.; Lee, Delphine J.; Freeman, William R.; Flores-Aguilar, Marisa; Spector, Stephen A.

doi:10.1172/jci117648

Cited by 129 publications

(74 citation statements)

References 24 publications

(30 reference statements)

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“…A591V has not been documented as a polymorphism in baseline UL97 sequences from untreated subjects but has occasionally been detected since the early use of GCV (5,20,21), including the emergence of A591V as a new mutation after GCV therapy (22). The first published phenotype was from plaque reduction assays showing a GCV EC 50 of 7.9 M, which was 1.3-fold increased over control wild-type EC 50 s (5) but above the cutoff of 6 M originally proposed for classifying GCV resistance (23).…”

Section: Discussionmentioning

confidence: 99%

Differentiated Levels of Ganciclovir Resistance Conferred by Mutations at Codons 591 to 603 of the Cytomegalovirus UL97 Kinase Gene

2017

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Diagnostic mutations in the cytomegalovirus UL97 kinase gene are used to assess the level of associated ganciclovir resistance and therapeutic options. The best-known mutations at codons 460, 520, or 591 to 607 individually confer 5-to 10-fold-decreased ganciclovir susceptibility, except that a 3-fold decrease occurs in the case of the amino acid substitution C592G. Less common point and in-frame deletion mutations at codons 591 to 603 remain incompletely characterized. The ganciclovir susceptibilities of 17 mutants in this codon range were evaluated by use of the same recombinant phenotyping system and extensive assay replicates in two types of cell cultures. Amino acid substitutions K599E and T601M conferred no ganciclovir resistance, while A591V conferred 3.8-fold-decreased susceptibility. In-frame deletions of three or more codons conferred at least 8-fold-increased ganciclovir resistance, while the level of resistance conferred by one-or two-codon deletions varied from 4-to 10-fold, depending on their location. Measured levels of ganciclovir resistance were closely comparable when assays were performed in either fibroblasts or modified retinal epithelial cells. The significant revision of a few previously published resistance phenotypes and the new data strengthen the interpretation of genotypic testing for cytomegalovirus drug resistance.KEYWORDS cytomegalovirus, drug resistance mechanisms, ganciclovir P rolonged treatment of human cytomegalovirus (CMV) infection with ganciclovir (GCV) or its oral prodrug, valganciclovir, may result in antiviral drug resistance when viral replication is incompletely suppressed. Without the routine availability of susceptibility testing on CMV culture isolates, the laboratory diagnosis of drug resistance is dependent on the direct detection of characteristic viral mutations in clinical specimens (1, 2). GCV resistance mutations usually develop first in the UL97 kinase gene involved in the initial phosphorylation of GCV that is necessary for its antiviral action. One of seven UL97 mutations (M460V/I, H520Q, C592G, A594V, L595S, and C603W) is initially detected in Ͼ80% of cases of GCV resistance in clinical practice, with most of the remainder consisting of less common amino acid substitutions or in-frame deletions at codons 590 to 607 or of mutations in the UL54 DNA polymerase gene (2). The canonical UL97 mutations confer 5-to 10-fold increases in the GCV concentration required for 50% viral growth inhibition (50% effective concentration [EC 50 ]), except that C592G confers a 3-fold increase. Given the limited alternative treatment options, mutations conferring lower-grade resistance may be amenable to GCV dose escalation, according to consensus treatment guidelines (3). Therefore, accurate calibration of the levels of resistance conferred by specific mutations is desirable for treatment planning purposes

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Section: Discussionmentioning

confidence: 99%

Differentiated Levels of Ganciclovir Resistance Conferred by Mutations at Codons 591 to 603 of the Cytomegalovirus UL97 Kinase Gene

2017

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“…This could indicate that this region might be involved in substrate binding. Point mutations and small deletions in this domain have been detected in phenotypically GCV-resistant HCMV (Lurain et al, 1994 ;Wolf et al, 1995 ;Baldanti et al, 1995 ;Chou et al, 1995 ;Hanson et al, 1995). The 4 aa deletion and the point mutations investigated here in the vaccinia virus system had no detectable influence on phosphorylation of pUL97.…”

Section: Cbbamentioning

confidence: 99%

“…which induce the resistance of HCMV strains to GCV in biological assays (Sullivan et al, 1992 ;Lurain et al, 1994 ;Wolf et al, 1995 ;Baldanti et al, 1995 ;Chou et al, 1995 ;Hanson et al, 1995). Until now, only point mutations between amino acids 460 and 607 have been detected in GCV-resistant clinical isolates, and neither isolation of clinical HCMV strains lacking the UL97 ORF or carrying extended deletions in the UL97 ORF has been reported, nor has anyone succeeded in generating such mutants in the laboratory (He et al, 1997 ;Michel et al, 1996).…”

Section: Introductionmentioning

confidence: 99%

Functional regions of the human cytomegalovirus protein pUL97 involved in nuclear localization and phosphorylation of ganciclovir and pUL97 itself.

Michel

Schaarschmidt

Wunderlich

et al. 1998

Journal of General Virology

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In order to identify functional regions of the human cytomegalovirus protein pUL97 (i) different 5h fragments of the UL97 open reading frame (ORF) were fused to the coding region of the green fluorescent protein and (ii) recombinant vaccinia viruses (rVV) were generated carrying two full-length and 11 mutated UL97 ORFs. The results indicated the presence of an N-terminal region within pUL97 which changed the intracellular distribution of the fusion proteins. pUL97 was localized in the nucleus, but not in the nucleoli, and was detected in the nuclear matrix fraction. Expression of all pUL97 mutants could be confirmed by Western blot analysis. pUL97-associated ganciclovir (GCV) phos-

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“…The facts, that specific mutations in the UL97 and UL54 genes are associated with antiviral drug resistance, have led to the development of genetic methods. These are based on PCR amplification of the specific region of the genome followed by restriction enzyme analysis or direct sequencing of the amplification product/products (Alain et al, 1997;Lurain et al, 2002;Mendez et al, 1999b;Wolf et al, 1995). An obvious advantage of these assays is the possibility to use clinical specimens directly, rather than virus isolates, which significantly shortens the time required for performance of the test.…”

Section: Laboratory Diagnosis Of Hcmvmentioning

confidence: 99%

Drug Resistance due to Mutation in UL 97 and Certain Other Specific Genes in Cytomegalovirus Strains: An Overview

Kumar¹

2013

IOSR-JPBS

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Mutations in human cytomegalovirus UL97 gene confer clinical resistance to ganciclovir and can be detected directly in patient plasma.

Cited by 129 publications

References 24 publications

Differentiated Levels of Ganciclovir Resistance Conferred by Mutations at Codons 591 to 603 of the Cytomegalovirus UL97 Kinase Gene

Differentiated Levels of Ganciclovir Resistance Conferred by Mutations at Codons 591 to 603 of the Cytomegalovirus UL97 Kinase Gene

Functional regions of the human cytomegalovirus protein pUL97 involved in nuclear localization and phosphorylation of ganciclovir and pUL97 itself.

Drug Resistance due to Mutation in UL 97 and Certain Other Specific Genes in Cytomegalovirus Strains: An Overview

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