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评估鸡肾和鸡胚肾培养物用于减毒流感病毒主毒株A/Ann/Arbor/6/60-ca的大规模生长。

Evaluation of chicken kidney and chicken embryo kidney cultures for the large-scale growth of attenuated influenza virus master strain A/Ann/Arbor/6/60-ca.

作者信息

Tannock G A, Bryce D A, Paul J A

出版信息

Vaccine. 1985 Sep;3(3):333-9.

PMID:4060843
Abstract

Primary chicken kidney (CK) and chicken embryo kidney (CEK) cells were evaluated as possible substrates for growth of the cold-adapted attenuated influenza vaccine master strain A/Ann Arbor/6/60 (A/AA/6/60-ca). Yields of 10(6)-10(7) TCID50 per ml of culture fluid were obtained in either cell type. Yields from the human diploid strain MRC-5 were approximately 100-fold less. More reproducible cultures were obtained from CEK cells, using an overnight trypsinization step at 4 degrees C, than from CK cells. Comparable yields per embryo were obtained from CEK cells grown in roller cultures to those grown on the surface of microcarriers. These yields were less than those obtained from the allantoic fluids of whole embryos. Frozen storage of CEK or CK cells, after primary trypsinization, dispersal from a cultured CK primary monolayer or culture on microcarriers, was unsuccessful. The cold-adapted phenotype of A/AA/6/60-ca was retained after growth in CEK cultures and no differences in immunogenicity were detectable in mice between CEK- and allantoic-grown virus. Allantoic-grown preparations of A/AA/6/60-ca contained a lower protein concentration per infectious unit than those grown in CEK.

摘要

对原代鸡肾(CK)细胞和鸡胚肾(CEK)细胞作为冷适应减毒流感疫苗主毒株A/Ann Arbor/6/60(A/AA/6/60-ca)生长的可能底物进行了评估。在这两种细胞类型中,每毫升培养液均获得了10⁶ - 10⁷半数组织培养感染剂量(TCID₅₀)的产量。人二倍体细胞株MRC-5的产量约低100倍。与CK细胞相比,通过在4℃过夜胰蛋白酶消化步骤,从CEK细胞获得的培养物更具重复性。在滚瓶培养中生长的CEK细胞与在微载体表面生长的CEK细胞相比,每个胚胎的产量相当。这些产量低于从全胚胎尿囊液中获得的产量。在原代胰蛋白酶消化、从培养的CK原代单层细胞分散或在微载体上培养后,对CEK或CK细胞进行冷冻保存均未成功。A/AA/6/60-ca在CEK培养物中生长后保留了冷适应表型,并且在小鼠中,CEK培养的病毒和尿囊液培养的病毒之间在免疫原性上没有可检测到的差异。A/AA/6/60-ca的尿囊液培养制剂每感染单位的蛋白质浓度低于在CEK中培养的制剂。

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