Analysis of hepatitis B virus-mixed genotype infection by ultra deep pyrosequencing in Sudanese patients, 2015-2016

被引:4
|
作者
Enan, Khalid Abdallah [1 ]
Minosse, Claudia [2 ]
El Hussein, Abdel Rahim Mohammed [1 ]
Selleri, Marina [2 ]
Giombini, Emanuela [2 ]
Capobianchi, Maria Rosaria [2 ]
Elkhidir, Isam Mohamed [3 ]
Mustafa, Mohamed Omer [1 ]
Khair, Osama Mohamed [3 ]
Hassan, Dina Ahamed [1 ]
Garbuglia, Anna Rosa [2 ]
机构
[1] Minist Higher Educ & Sci Res, Cent Lab, Dept Virol, Khartoum 7099, Sudan
[2] Natl Inst Infect Dis Lazzaro Spallanzani IRCCS, Virol Lab, Via Portuense 292, I-00149 Rome, Italy
[3] Univ Khartoum, Fac Med, Dept Microbiol & Parasitol, Khartoum 7099, Sudan
关键词
Hepatitis B virus; High-throughput nucleotide sequencing; Sudan; Co-infection; LINE PROBE ASSAY; INNO-LIPA HBV; MOLECULAR CHARACTERIZATION; BLOOD-DONORS; LAMIVUDINE; SEQUENCE; STRAINS; SUBGENOTYPES; COINFECTION; VARIABILITY;
D O I
10.1007/s15010-019-01306-5
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
Purpose The frequency of detection of HBV co-infection with multiple HBV genotypes is influenced by the detection method; usually co-infections are detected by multiplex PCR or hybridization assays, and are rarely confirmed by sequencing and conventional cloning. The objective of this study was to confirm by ultra-deep pyrosequencing (UDPS) mixed HBV infections, previously detected by multiplex-nested PCR. Methods Sixteen samples from HBV co-infected Sudanese patients detected by multiplex-nested PCR, were amplified targeting the P/S region and sequenced by UDPS. Results The only genotypes identified using UDPS were D and E, while A, B, C and F genotypes, previously detected by multiplex-nested PCR, were not detected. Specifically, 10 samples were shown to be mono-infected (D or E); in 3 out of 10 mono-infected D patients, a subtype combination was observed: D1 + D7 in 2 cases and D2 + D6 in 1 case. The remaining 6 subjects were D + E co-infected (harboring different mixtures of D subtypes). Conclusions Overall, UDPS is more effective than multiplex-nested PCR for identifying multiple HBV genotypes and subtypes infections.
引用
收藏
页码:793 / 803
页数:11
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