Klimstra W B, Ryman K D, Johnston R E
Department of Microbiology and Immunology, School of Medicine, University of North Carolina at Chapel Hill, Chapel Hill, North Carolina, USA.
J Virol. 1998 Sep;72(9):7357-66. doi: 10.1128/JVI.72.9.7357-7366.1998.
Attachment of Sindbis virus to the cell surface glycosaminoglycan heparan sulfate (HS) and the selection of this phenotype by cell culture adaptation were investigated. Virus (TR339) was derived from a cDNA clone representing the consensus sequence of strain AR339 (K. L. McKnight, D. A. Simpson, S. C. Lin, T. A. Knott, J. M. Polo, D. F. Pence, D. B. Johannsen, H. W. Heidner, N. L. Davis, and R. E. Johnston, J. Virol. 70:1981-1989, 1996) and from mutant clones containing either one or two dominant cell culture adaptations in the E2 structural glycoprotein (Arg instead of Ser at E2 position 1 [designated TRSB]) or this mutation plus Arg for Ser at E2 114 [designated TRSB-R114]). The consensus virus, TR339, bound to baby hamster kidney (BHK) cells very poorly. The mutation in TRSB increased binding 10- to 50-fold, and the additional mutation in TRSB-R114 increased binding 3- to 5-fold over TRSB. The magnitude of binding was positively correlated with the degree of cell culture adaptation and with attenuation of these viruses in neonatal mice. HS was identified as the attachment receptor for the mutant viruses by the following experimental results. (i) Low concentrations of soluble heparin inhibited plaque formation on and binding of mutant viruses to BHK cells by >95%. In contrast, TR339 showed minimal inhibition at high concentrations. (ii) Binding and infectivity of TRSB-R114 was sensitive to digestion of cell surface HS with heparinase III, and TRSB was sensitive to both heparinase I and heparinase III. TR339 infectivity was only slightly affected by either digestion. (iii) Radiolabeled TRSB and TRSB-R114 attached efficiently to heparin-agarose beads in binding assays, while TR339 showed virtually no binding. (iv) Binding and infectivity of TRSB and TRSB-R114, but not TR339, were greatly reduced on Chinese hamster ovary cells deficient in HS specifically or all glycosaminoglycans. (v) High-multiplicity-of-infection passage of TR339 on BHK cell cultures resulted in rapid coselection of high-affinity binding to BHK cells and attachment to heparin-agarose beads. Sequencing of the passaged virus population revealed a mutation from Glu to Lys at E2 70, a mutation common to many laboratory strains of Sindbis virus. These results suggest that TR339, the most virulent virus tested, attaches to cells through a low-affinity, primarily HS-independent mechanism. Adaptive mutations, selected during cell culture growth of Sindbis virus, enhance binding and infectivity by allowing the virus to attach by an alternative mechanism that is dependent on the presence of cell surface HS.
研究了辛德毕斯病毒与细胞表面糖胺聚糖硫酸乙酰肝素(HS)的结合以及通过细胞培养适应性选择该表型的情况。病毒(TR339)源自一个代表AR339株(K. L. 麦克奈特、D. A. 辛普森、S. C. 林、T. A. 诺特、J. M. 波罗、D. F. 彭斯、D. B. 约翰森、H. W. 海德纳、N. L. 戴维斯和R. E. 约翰斯顿,《病毒学杂志》70:1981 - 1989,1996)一致序列的cDNA克隆,以及来自在E2结构糖蛋白中含有一个或两个显性细胞培养适应性突变的突变克隆(E2位置1处为精氨酸而非丝氨酸[命名为TRSB])或该突变加上E2 114处的精氨酸替代丝氨酸[命名为TRSB - R114])。一致病毒TR339与幼仓鼠肾(BHK)细胞的结合非常差。TRSB中的突变使结合增加了10至50倍,TRSB - R114中的额外突变使结合比TRSB增加了3至5倍。结合程度与细胞培养适应性程度以及这些病毒在新生小鼠中的减毒程度呈正相关。通过以下实验结果确定HS为突变病毒的附着受体。(i)低浓度的可溶性肝素抑制突变病毒在BHK细胞上形成噬斑以及与BHK细胞的结合>95%。相比之下,TR339在高浓度时显示出最小抑制。(ii)TRSB - R114的结合和感染性对用肝素酶III消化细胞表面HS敏感,而TRSB对肝素酶I和肝素酶III均敏感。TR339的感染性仅受到两种消化的轻微影响。(iii)在结合试验中,放射性标记的TRSB和TRSB - R114有效地附着于肝素 - 琼脂糖珠,而TR339几乎没有结合。(iv)在特异性缺乏HS或所有糖胺聚糖的中国仓鼠卵巢细胞上,TRSB和TRSB - R114的结合和感染性,但不是TR339的,大大降低。(v)TR339在BHK细胞培养物上的高感染复数传代导致快速共选择与BHK细胞的高亲和力结合以及附着于肝素 - 琼脂糖珠。传代病毒群体的测序揭示了E2 70处从谷氨酸到赖氨酸的突变,这是许多辛德毕斯病毒实验室菌株共有的突变。这些结果表明,测试的最具毒力的病毒TR339通过低亲和力、主要不依赖HS的机制附着于细胞。在辛德毕斯病毒的细胞培养生长过程中选择的适应性突变通过允许病毒通过依赖细胞表面HS存在的替代机制附着来增强结合和感染性。
