Yao Q Y, Tierney R J, Croom-Carter D, Cooper G M, Ellis C J, Rowe M, Rickinson A B
CRC Institute for Cancer Studies, University of Birmingham, United Kingdom.
J Virol. 1996 Aug;70(8):4895-903. doi: 10.1128/JVI.70.8.4895-4903.1996.
All wild-type isolates of Epstein-Barr virus (EBV) analyzed to date for allelic polymorphisms of the nuclear antigen EBNA2 gene (in the BamHI YH region of the genome) and of the EBNA3A,-3B, -3C genes (tandemly arranged in the BamHI E region) have proved either uniformly type 1 or uniformly type 2 at all four loci. The absence of detectable intertypic recombination in the wild probably reflects the rarity with which individual carriers, and certainly individual target cells, become coinfected with both virus types. Studying a group of human immunodeficiency virus-positive T-cell-immunocompromised patients known to be at enhanced risk of multiple EBV infections, we have isolated intertypic EBV recombinants from 2 of 40 patients analyzed. These recombinants, whose in vitro transforming capacity appeared at least equal to that of type 1 strains, carried a type 1 EBNA2 allele and type 2 EBNA3A,-3B, and -3C alleles. This was clearly demonstrable at the DNA level by PCR amplification using type-specific primer-probe combinations and was confirmed at the protein level (for EBNA2 and EBNA3C) by immunoblotting with type-specific antibodies. In one patient, the recombinant appeared to be the predominant strain, being the virus most commonly rescued by in vitro transformation both from the blood and from the throat washings on two separate occasions 20 months apart. A regular type 1 virus strain was also present in this individual, but this was not related to the recombinant since the two viruses carried type 1 EBNA2 genes with different patterns of variance from the B95.8 prototype sequence. In the other patient, recombinants were isolated on one occasion from the blood and on a separate occasion, 21 months later, from the throat; these recombinants were almost certainly related, being identical at several genomic polymorphisms and differing only in one facet of the "EBNAprint," the size of the EBNA1 protein. Three different type 1 viruses were also isolated from this patient, two of which carried EBNA2 genes with the same pattern of sequence variation from B95.8 as the recombinant; however, since this is a fairly common pattern of variance, the relationship of these viruses to the recombinant remains an open question. We infer that intertypic recombinants of EBV are not uncommon in HIV-positive T-cell-immunocompromised patients, that they arise in such individuals as a consequence of their increased frequency of mixed-type infections, and that they will prove capable of efficient transmission in the human population.
迄今为止,对所有经分析的爱泼斯坦 - 巴尔病毒(EBV)野生型分离株的核抗原EBNA2基因(在基因组的BamHI YH区域)以及EBNA3A、-3B、-3C基因(串联排列在BamHI E区域)的等位基因多态性研究表明,在所有这四个位点上,它们要么均为1型,要么均为2型。野生状态下未检测到型间重组现象,这可能反映出个体携带者,当然还有单个靶细胞,同时感染两种病毒类型的情况极为罕见。在研究一组已知有更高风险发生多次EBV感染的人类免疫缺陷病毒阳性且T细胞免疫受损的患者时,我们从40名接受分析的患者中的2名患者体内分离出了型间EBV重组体。这些重组体在体外的转化能力似乎至少与1型毒株相当,它们携带1型EBNA2等位基因以及2型EBNA3A、-3B和-3C等位基因。通过使用型特异性引物 - 探针组合进行PCR扩增,在DNA水平上清晰地证实了这一点,并且通过用型特异性抗体进行免疫印迹分析,在蛋白质水平(针对EBNA2和EBNA3C)上也得到了证实。在一名患者中,重组体似乎是主要毒株,在两次相隔20个月的不同时间,它都是通过体外转化从血液和咽洗液中最常分离出的病毒。该个体中也存在一种常规的1型病毒株,但它与重组体无关,因为这两种病毒携带的1型EBNA2基因与B95.8原型序列的变异模式不同。在另一名患者中,一次从血液中分离出重组体,21个月后又从咽部分离出重组体;这些重组体几乎可以肯定是相关的,它们在几个基因组多态性位点上相同,只是在“EBNA指纹”的一个方面有所不同,即EBNA1蛋白的大小。从该患者体内还分离出了三种不同的1型病毒,其中两种携带的EBNA2基因与重组体具有相同的相对于B95.8的序列变异模式;然而,由于这是一种相当常见的变异模式,这些病毒与重组体之间的关系仍有待确定。我们推断,EBV的型间重组体在HIV阳性且T细胞免疫受损的患者中并不罕见,它们在这类个体中出现是由于混合感染频率增加的结果,并且它们将被证明能够在人群中有效传播。
