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四种呼吸道合胞病毒蛋白的纯化及其作为抗BALB/c小鼠实验性感染保护剂的评估。

The purification of four respiratory syncytial virus proteins and their evaluation as protective agents against experimental infection in BALB/c mice.

作者信息

Routledge E G, Willcocks M M, Samson A C, Morgan L, Scott R, Anderson J J, Toms G L

机构信息

Department of Virology, University of Newcastle upon Tyne, U.K.

出版信息

J Gen Virol. 1988 Feb;69 ( Pt 2):293-303. doi: 10.1099/0022-1317-69-2-293.

Abstract

The fusion (F) glycoprotein, large glyco- (G) protein, phospho- (P) protein and 22K protein of respiratory syncytial (RS) virus A2 strain were purified by a combination of immunoaffinity adsorption and preparative SDS-PAGE. All four proteins elicited serum antibody in mice after repeated inoculation in adjuvant, although the magnitude of the response as measured by ELISA varied from mouse to mouse. The F protein generated neutralizing antibodies in only 50% of the mice determined to be seropositive by ELISA. The G protein also induced neutralizing antibodies but in this instance neutralization tests and ELISA titres were more closely correlated. No neutralizing activity was detected in mice immunized with the P or 22K proteins although all produced antibody detectable by ELISA. Mice immunized with either the F or the G protein were found to be protected against subsequent RS virus challenge, whether they had developed neutralizing antibody or not. Mice inoculated with the P or 22K proteins were not protected.

摘要

呼吸道合胞病毒A2株的融合(F)糖蛋白、大糖蛋白(G)、磷蛋白(P)和22K蛋白通过免疫亲和吸附和制备性SDS-PAGE相结合的方法进行纯化。在佐剂中反复接种后,所有这四种蛋白均能在小鼠体内诱导血清抗体产生,尽管通过ELISA测定的反应强度在不同小鼠之间有所差异。通过ELISA测定为血清阳性的小鼠中,只有50%的小鼠在接种F蛋白后产生了中和抗体。G蛋白也诱导产生了中和抗体,但在这种情况下,中和试验和ELISA滴度的相关性更强。在用P蛋白或22K蛋白免疫的小鼠中未检测到中和活性,尽管所有小鼠均产生了可通过ELISA检测到的抗体。发现用F蛋白或G蛋白免疫的小鼠,无论是否产生了中和抗体,均能抵抗随后的呼吸道合胞病毒攻击。接种P蛋白或22K蛋白的小鼠未得到保护。

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