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通过酶免疫测定法检测包括猴疱疹病毒在内的灵长类疱疹病毒抗体。

Detection of primate herpesvirus antibodies including Herpesvirus simiae by enzyme immunoassay.

作者信息

Eichberg J W, Heberling R L, Guajardo J E, Kalter S S

出版信息

Dev Biol Stand. 1980;45:61-6.

PMID:6249690
Abstract

An enzyme immunoassay (EIA) was used for the detection of antibodies to Herpesvirus hominis type 1 and 2 (HVH-1 and HVH-2), SA8 and Herpesvirus simiae (HVB) in human and nonhuman primate sera. Optimal assay conditions were approximately the same for HVH-1, HVH-2, and SA8 but different for HVB. The recognized lethality of HVB required studies to determine whether or not inactivated HVB could be used in the EIA outside a biohazard safety cabinet. Ten percent buffered formalin destroyed infectivity of antigen coated discs after 5 minutes while retaining activity in the EIA. Antibody titers to HVB determined by serum neutralization were up to eightfold higher in the EIA. Using EIA to survey sera for antibodies to herpesviruses, it was determined that most humans reacted to HVH-1 (88%), HVH-2 (81%) and SA8 (94%), and 38% to HVB. Whereas baboons reacted almost exclusively to their indigenous herpesvirus SA8 (44%), rhesus monkeys demonstrated a high positive rate to HVH-1 (63%), SA8 (94%), and HVB (50%). These data indicate that EIA is rapid, sensitive, reproducible, and useful in the detection of antibodies to human and nonhuman primate herpesviruses but does not, at this point, resolve problems related to cross-reactivity among these viruses.

摘要

采用酶免疫测定法(EIA)检测人和非人灵长类动物血清中1型和2型人疱疹病毒(HVH - 1和HVH - 2)、SA8病毒及猴疱疹病毒(HVB)的抗体。HVH - 1、HVH - 2和SA8的最佳测定条件大致相同,但HVB的测定条件不同。鉴于HVB具有公认的致死性,需要开展研究以确定在生物安全柜外进行EIA检测时,灭活的HVB是否可用。10%的缓冲甲醛在5分钟后可破坏包被抗原的圆盘的感染性,但在EIA中仍保留活性。通过血清中和法测定的针对HVB的抗体效价在EIA中高出多达八倍。利用EIA检测血清中的疱疹病毒抗体,结果显示大多数人对HVH - 1(88%)、HVH - 2(81%)和SA8(94%)有反应,对HVB有反应的占38%。狒狒几乎只对其本土疱疹病毒SA8有反应(44%),而恒河猴对HVH - 1(63%)、SA8(94%)和HVB(50%)呈现出较高的阳性率。这些数据表明,EIA在检测人和非人灵长类动物疱疹病毒抗体方面快速、灵敏、可重复且有用,但目前尚不能解决这些病毒之间交叉反应相关的问题。

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