马传染性贫血病毒体内致病分子克隆的构建与特性分析
Development and characterization of an in vivo pathogenic molecular clone of equine infectious anemia virus.
作者信息
Cook R F, Leroux C, Cook S J, Berger S L, Lichtenstein D L, Ghabrial N N, Montelaro R C, Issel C J
机构信息
Department of Veterinary Science, Gluck Equine Research Center, University of Kentucky, Lexington 40546, USA.
出版信息
J Virol. 1998 Feb;72(2):1383-93. doi: 10.1128/JVI.72.2.1383-1393.1998.
An infectious nonpathogenic molecular clone (19-2-6A) of equine infectious anemia virus (EIAV) was modified by substitution of a 3.3-kbp fragment amplified by PCR techniques from a pathogenic variant (EIAV(PV)) of the cell culture-adapted strain of EIAV (EIAV(PR)). This substitution consisted of coding sequences for 77 amino acids at the carboxyl terminus of the integrase, the S1 (encoding the second exon of tat), S2, and S3 (encoding the second exon of rev) open reading frames, the complete env gene (including the first exon of rev), and the 3' long terminal repeat (LTR). Modified 19-2-6A molecular clones were designated EIAV(PV3.3), and infection of a single pony (678) with viruses derived from a mixture of five of these molecular clones induced clinical signs of acute equine infectious anemia (EIA) at 23 days postinfection (dpi). As a consequence of this initial study, a single molecular clone, EIAV(PV3.3#3) (redesignated EIAV(UK)), was selected for further study and inoculated into two ponies (613 and 614) and two horses (700 and 764). Pony 614 and the two horses developed febrile responses by 12 dpi, which was accompanied by a 48 to 64% reduction in platelet number, whereas pony 613 did not develop fever (40.6 degrees C) until 76 dpi. EIAV could be isolated from the plasma of these animals by 5 to 7 dpi, and all became seropositive for antibodies to this virus by 21 dpi. Analysis of the complete nucleotide sequence demonstrated that the 3.3-kbp 3' fragment of EIAV(UK) differed from the consensus sequence of EIAV(PV) by just a single amino acid residue in the second exon of the rev gene. Complete homology with the EIAV(PV) consensus sequence was observed in the hypervariable region of the LTR. However, EIAV(UK) was found to contain an unusual 68-bp nucleotide insertion/duplication in a normally conserved region of the LTR sequence. These results demonstrate that substitution of a 3.3-kbp fragment from the EIAV(PV) strain into the infectious nonpathogenic molecular clone 19-2-6A leads to the production of progeny virus particles with the ability to induce clinical signs of EIA. Therefore, EIAV(UK), which is the first pathogenic, cell culture-adapted molecular clone of EIAV to be described, should be of value in identifying viral determinants of pathogenicity.
马传染性贫血病毒(EIAV)的一个感染性非致病性分子克隆(19 - 2 - 6A)通过用PCR技术从EIAV细胞培养适应株(EIAV(PR))的致病性变体(EIAV(PV))扩增得到的一个3.3 kbp片段进行替换而被修饰。该替换包括整合酶羧基末端77个氨基酸的编码序列、S1(编码tat的第二个外显子)、S2和S3(编码rev的第二个外显子)开放阅读框、完整的env基因(包括rev的第一个外显子)以及3'长末端重复序列(LTR)。修饰后的19 - 2 - 6A分子克隆被命名为EIAV(PV3.3),用源自这五个分子克隆混合物的病毒感染一匹小马(678),在感染后23天(dpi)引发了急性马传染性贫血(EIA)的临床症状。作为这项初步研究的结果,选择了一个单一的分子克隆EIAV(PV3.3#3)(重新命名为EIAV(UK))进行进一步研究,并接种到两匹小马(613和614)和两匹马(700和764)体内。小马614和两匹马在12 dpi时出现发热反应,同时血小板数量减少48%至64%,而小马613直到76 dpi才出现发热(40.6摄氏度)。在5至7 dpi时可从这些动物的血浆中分离出EIAV,到21 dpi时所有动物对该病毒的抗体均呈血清阳性。对完整核苷酸序列的分析表明,EIAV(UK)的3.3 kbp 3'片段与EIAV(PV)的共有序列仅在rev基因的第二个外显子中有一个氨基酸残基不同。在LTR的高变区观察到与EIAV(PV)共有序列完全同源。然而,发现EIAV(UK)在LTR序列的一个正常保守区域含有一个不寻常的68 bp核苷酸插入/重复。这些结果表明,将EIAV(PV)株的一个3.3 kbp片段替换到感染性非致病性分子克隆19 - 2 - 6A中会导致产生具有诱导EIA临床症状能力的子代病毒颗粒。因此,EIAV(UK)作为第一个被描述的致病性、细胞培养适应的EIAV分子克隆,在鉴定致病性病毒决定因素方面应该具有价值。
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