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1型人类免疫缺陷病毒(HIV)B亚型Tat蛋白在意大利、乌干达和南非HIV-1感染者中的序列保守性及抗体交叉识别

Sequence conservation and antibody cross-recognition of clade B human immunodeficiency virus (HIV) type 1 Tat protein in HIV-1-infected Italians, Ugandans, and South Africans.

作者信息

Buttò Stefano, Fiorelli Valeria, Tripiciano Antonella, Ruiz-Alvarez Maria J, Scoglio Arianna, Ensoli Fabrizio, Ciccozzi Massimo, Collacchi Barbara, Sabbatucci Michela, Cafaro Aurelio, Guzmán Carlos A, Borsetti Alessandra, Caputo Antonella, Vardas Eftyhia, Colvin Mark, Lukwiya Matthew, Rezza Giovanni, Ensoli Barbara

机构信息

Laboratory of Virology, Istituto Superiore di Sanità, University of Rome "La Sapienza," Rome, Italy.

出版信息

J Infect Dis. 2003 Oct 15;188(8):1171-80. doi: 10.1086/378412. Epub 2003 Sep 30.

DOI:10.1086/378412
PMID:14551888
Abstract

We determined immune cross-recognition and the degree of Tat conservation in patients infected by local human immunodeficiency virus (HIV) type 1 strains. The data indicated a similar prevalence of total and epitope-specific anti-Tat IgG in 578 serum samples from HIV-infected Italian (n=302), Ugandan (n=139), and South African (n=137) subjects, using the same B clade Tat protein that is being used in vaccine trials. In particular, anti-Tat antibodies were detected in 13.2%, 10.8%, and 13.9% of HIV-1-infected individuals from Italy, Uganda, and South Africa, respectively. Sequence analysis results indicated a high similarity of Tat from the different circulating viruses with BH-10 Tat, particularly in the 1-58 amino acid region, which contains most of the immunogenic epitopes. These data indicate an effective cross-recognition of a B-clade laboratory strain-derived Tat protein vaccine by individuals infected with different local viruses, owing to the high similarity of Tat epitopes.

摘要

我们测定了感染当地1型人类免疫缺陷病毒(HIV)毒株患者的免疫交叉识别情况以及Tat蛋白的保守程度。数据显示,在来自意大利(n = 302)、乌干达(n = 139)和南非(n = 137)的578份HIV感染患者血清样本中,使用疫苗试验中正在使用的同一B亚型Tat蛋白,总抗Tat IgG和表位特异性抗Tat IgG的流行率相似。具体而言,分别在13.2%、10.8%和13.9%的意大利、乌干达和南非HIV-1感染个体中检测到抗Tat抗体。序列分析结果表明,不同流行病毒的Tat蛋白与BH-10 Tat高度相似,尤其是在1 - 58氨基酸区域,该区域包含了大部分免疫原性表位。这些数据表明,由于Tat表位的高度相似性,感染不同当地病毒的个体对B亚型实验室毒株来源的Tat蛋白疫苗具有有效的交叉识别。

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