Typing of human rotaviruses: Nucleotide mismatches between the VP7 gene and primer are associated with genotyping failure

被引:25
作者
Rahman, Mustafizur [1 ,2 ]
Sultana, Rasheda [1 ]
Podder, Goutam [1 ]
Faruque, Abu S. G. [1 ]
Matthijnssens, Jelle [2 ]
Zaman, Khalequz [1 ]
Breiman, Robert F. [1 ]
Sack, David A. [1 ]
Van Ranst, Marc [2 ]
Azim, Tasnim [1 ]
机构
[1] ICDDR B, Ctr Hlth & Populat Res B, Dhaka 1212, Bangladesh
[2] Katholieke Univ Leuven, Rega Inst Med Res, Lab Clin & Epidemiol Virol, B-3000 Louvain, Belgium
关键词
Stool Specimen; Hyperimmune Antiserum; Untypeable Strain; Sandwich Type Enzyme Immunoassay; Dhaka Hospital;
D O I
10.1186/1743-422X-2-24
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Background: Rotavirus genotyping is performed by using reverse transcription PCR with type-specific-primers. Because the high rotavirus mutation rate generates an extensive genomic variation, different G-type-specific primer sets are applied in different geographical locations. In Bangladesh, a significant proportion (36.9%) of the rotavirus strains isolated in 2002 could not be G-typed using the routinely used primer set. To investigate the reason why the strains were untypeable, nucleotide sequencing of the VP7 genes was performed. Results: Four nucleotide substitutions at the G1 primer-binding site of the VP7 gene of Bangladeshi G1 rotaviruses rendered a major proportion of circulating strains untypeable using the routine primer set. Using an alternative primer set, we could identify G1 rotaviruses as the most prevalent genotype (44.8%), followed by G9 (21.7%), G2 (15.0%) and G4 (13.8%). Conclusion: Because of the natural variation in the rotaviral gene sequences, close monitoring of rotavirus genotyping methods is important.
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页数:5
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