Susceptibility to AcMNPV and Expression of Recombinant Proteins by a Novel Cell Clone Derived from a Trichoplusia ni QAU-BTI-Tn9-4s Cell Line 被引量：1

Susceptibility to AcMNPV and Expression of Recombinant Proteins by a Novel Cell Clone Derived from a Trichoplusia ni QAU-BTI-Tn9-4s Cell Line

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摘要 It is well known that Tn5B1-4 (commercially known as the High Five) cell line is highly susceptible to baculovirus and provides superior production of recombinant proteins when compared to other insect cell lines.But the characteristics of the cell line do not always remain stable and may change upon continuous passage.Recently an alphanodavirus,named Tn5 Cell Line Virus (or TNCL Virus),was identified in High Five cells in particular.Therefore,we established a new cell line,QB-Tn9-4s,from Trichoplusia ni,which was determined to be free of TNCL virus by RT-PCR analysis.In this paper,we describe the development of a novel cell clone,QB-CL-B,from a low passage QB-Tn9-4s cell line and report its susceptibility to AcMNPV,and the level of recombinant protein production.This cell clone was similar to its parental cells QB-Tn9-4s and Tn5B1-4 cells in morphology and growth rate;although it also showed approximately the same responses to AcMNPV infection and production of occlusion bodies,there were higher levels of recombinant protein production in comparison to QB-Tn9-4s (parental cells) and High5 cells. It is well known that Tn5B1-4 （commercially known as the High Five） cell line is highly susceptible to baculovirus and provides superior production of recombinant proteins when compared to other insect cell lines. But the characteristics of the cell line do not always remain stable and may change upon continuous passage. Recently an alphanodavirus, named Tn5 Cell Line Virus （or TNCL Virus）, was identified in High Five cells in particular. Therefore, we established a new cell line, QB-Tn9-4s, from Trichoplusia ni, which was determined to be free of TNCL virus by RT-PCR analysis. In this paper, we describe the development of a novel cell clone, QB-CL-B, from a low passage QB-Tn9-4s cell line and report its susceptibility to AcMNPV, and the level of recombinant protein production. This cell clone was similar to its parental cells QB-Tn9-4s and Tn5B1-4 cells in morphology and growth rate; although it also showed approximately the same responses to AcMNPV infection and production of occlusion bodies, there were higher levels of recombinant protein production in comparison to QB-Tn9-4s （parental cells） and High5 cells.

作者 Ming Shan Shi-ying Zhang Lei Jiang Ming Ma Guo-xun Li

机构地区 A Center for Advanced Invertebrate Cell Engineering Collaborated Between Boyce Thompson Institute and Qingdao Agricultural University Boyce Thompson Institute （BTI） at Cornell University

出处《Virologica Sinica》 SCIE CAS CSCD 2011年第5期297-305,共9页 中国病毒学（英文版）

基金 supported in part by the Chinese National Basic Research Program(973)2009CB118900 Chinese National Science Foundation Project30771451 Boyce Thompson Institute Project BTI-QAU1-23-2007

关键词 ACMNPV 细胞克隆重组蛋白 NI 敏感性 BTI 昆虫细胞系杆状病毒 Cell line Insect virus Recombinant protein expression RT-PCR TNCL virus

分类号 Q939.4 [生物学—微生物学] Q785 [生物学—分子生物学]

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