摘要
目的分析TTV(Transfusiontransmitedvirus)深圳分离株ORF1部分基因序列。方法在TTVORF1设计引物,建立巢式聚合酶链反应(Nested-PCR),检测40例广东地区非甲-庚型肝炎患者血清中TTVDNA。对PCR产物进行分子克隆,以荧光法(AppliedBiosystems,373A)测序。结果40例非甲-庚型肝炎中21例TTVDNA阳性(52.5%)。对其中一株TTV(SZ1)ORF1部分基因克隆、测序,并与Okamoto等报道的2株(N22、G1a)相比较,其核苷酸序列的同源性分别为96.7%与97.4%。结论本研究证实我国华南地区存在TTV感染。
Objective To analyse partial nucleotide sequence of ORF 1 of TTV (transfusion transmitted virus) isolated from a patient with non A G hepatitis in Shenzhen. Methods A nested polymerase chain reaction (PCR) assay with primers from ORF 1 of TTV genome was established to detect TTV DNA in 40 patients with non A G hepatitis in Guangdong.PCR product was cloned and sequenced with the Applied Biosystems (373A). Results TTV DNA was positive in 21 of 40 patients (52.5%) with non A G hepatitis.Partial gene of ORF 1 of a TTV isolate (SZ1) was cloned,sequenced and compared with known sequences of TTV isolates (N22,G1a) reported by Okamoto.The nucleotide homology were 96.7% between SZ1 and N22,97.4% between SZ1 and G1a.Conclusion The results of this study confirmed the epidemic of TTV infection in Southern China.The cloning and sequencing of the TTV isolate (SZ1) and the development of a PCR assay for detecting TTV DNA has important implication for the diagnosis and epidemiological investigation on TTV infection.
出处
《中华传染病杂志》
CAS
CSCD
北大核心
1998年第3期131-133,共3页
Chinese Journal of Infectious Diseases
基金
深圳市优秀青年科技人才基金
