Williams M V, Parris D S
Virology. 1987 Feb;156(2):282-92. doi: 10.1016/0042-6822(87)90408-9.
The herpes simplex virus type 2 (HSV-2)-induced deoxyuridine triphosphate nucleotidohydrolase (dUTPase) was purified approximately 600 +/- 43-fold using a combination of affinity, hydrophobic, absorption, and ion-exchange chromatography techniques. The only substrate for the dUTPase was dUTP with a Km of 3.6 +/- 1.1 microM. There was no apparent divalent cation requirement, but the HSV-2-induced dUTPase was inhibited by EDTA (0.1 mM) and this inhibition was reversed by either Co2+ (0.5 mM) or Mg2+ (0.5 mM). The HSV-2-induced dUTPase was distinguished from the HSV-1-induced and cellular dUTPases based upon differences in sensitivity to substrate inhibition, thermostability, and electrophoretic migration in nondenaturing polyacrylamide gels. Analysis of HSV-1 temperature-sensitive (ts) mutants demonstrated that ts A15 and ts K13 did not induce significant amounts of dUTPase activity at the permissive or nonpermissive temperatures. Mutants with defects in HSV-induced DNA polymerase or in the major DNA binding protein induced dUTPase at both temperatures. In contrast ts mutants defective in the alpha polypeptide VP175 (ICP4) did not induce normal levels of dUTPase at the nonpermissive temperature. The location of a gene encoding for the type specificity of the HSV induced dUTPase was mapped to the left 20% of the genome in Us in the region 0.060 to 0.100 or from 0.148 to 0.204.
利用亲和色谱、疏水色谱、吸附色谱和离子交换色谱技术相结合的方法,将2型单纯疱疹病毒(HSV - 2)诱导的脱氧尿苷三磷酸核苷酸水解酶(dUTPase)纯化了约600±43倍。dUTPase的唯一底物是dUTP,其Km值为3.6±1.1微摩尔。该酶对二价阳离子无明显需求,但HSV - 2诱导的dUTPase受到EDTA(0.1毫摩尔)的抑制,而这种抑制作用可被Co2 +(0.5毫摩尔)或Mg2 +(0.5毫摩尔)逆转。基于对底物抑制的敏感性、热稳定性以及在非变性聚丙烯酰胺凝胶中的电泳迁移率差异,HSV - 2诱导的dUTPase与HSV - 1诱导的及细胞dUTPase得以区分。对HSV - 1温度敏感(ts)突变体的分析表明,ts A15和ts K13在允许温度或非允许温度下均未诱导出大量dUTPase活性。在HSV诱导的DNA聚合酶或主要DNA结合蛋白方面存在缺陷的突变体在这两个温度下均能诱导dUTPase。相比之下,在α多肽VP175(ICP4)方面存在缺陷的ts突变体在非允许温度下不能诱导出正常水平的dUTPase。编码HSV诱导的dUTPase类型特异性的基因定位在基因组左侧20%的Us区域,范围是0.060至0.100或0.148至0.204。
