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阿昔洛韦诱导兔角膜细胞中单纯疱疹病毒1型复制受抑制的分子分析

Molecular analysis of acyclovir-induced suppression of HSV-1 replication in rabbit corneal cells.

作者信息

Rong B L, Dunkel E C, Pavan-Langston D

机构信息

Eye Research Institute, Boston, Massachusetts 02114.

出版信息

Invest Ophthalmol Vis Sci. 1988 Jun;29(6):928-32.

PMID:2836333
Abstract

An in vitro HSV drug-suppression model has been established in rabbit corneal cell (SIRC) monolayers. Confluent SIRC monolayers were inoculated with McKrae strain HSV-1 (0.014 PFU/cell) and subsequently suppressed with acyclovir (ACV) (40 micrograms/ml) after adsorption for 1 hr at 37 degrees C. On days 0-5 postinoculation (PI), infectious HSV-1 was detected in approximately 50% of the SIRC cell cultures by standard supernatant and cell-free homogenate co-culture assays. On days 6-10 postsuppression, infectious HSV was detected in only 7-19% of the cultures. After removal of ACV suppression in the cultures (day 11 PI), HSV cytopathology developed to a 3-4+ level within 2-5 days. Dot blot hybridization of DNA extracted from the cultures indicated that the HSV genome was retained consistently in SIRC cells at a level of 0.0015-0.015 copies per cell during active ACV-suppression. During ACV-suppressed infection, approximately 0.9% of the SIRC cells contained the HSV genome as demonstrated by blot hybridization. After removal of ACV, a 1000-fold increase in HSV DNA concentration in SIRC cell cultures was detected.

摘要

已在兔角膜细胞(SIRC)单层中建立了体外单纯疱疹病毒(HSV)药物抑制模型。将汇合的SIRC单层接种McKrae株HSV-1(0.014空斑形成单位/细胞),然后在37℃吸附1小时后用阿昔洛韦(ACV)(40微克/毫升)进行抑制。在接种后(PI)0至5天,通过标准的上清液和无细胞匀浆共培养试验,在约50%的SIRC细胞培养物中检测到感染性HSV-1。在抑制后6至10天,仅在7%至19%的培养物中检测到感染性HSV。在培养物中去除ACV抑制后(接种后第11天),HSV细胞病变在2至5天内发展到3 - 4+级。从培养物中提取的DNA的斑点印迹杂交表明,在ACV有效抑制期间,HSV基因组在SIRC细胞中始终以每个细胞0.0015至0.015个拷贝的水平保留。在ACV抑制感染期间,如印迹杂交所示,约0.9%的SIRC细胞含有HSV基因组。去除ACV后,检测到SIRC细胞培养物中HSV DNA浓度增加了1000倍。

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