ADAM10和ADAM17在不同刺激物介导的CD16b脱落中的作用。

Sha Guo, Min Peng, Qing Zhao, Wei Zhang
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引用次数: 0

摘要

目的:探讨在不同刺激条件下CD16b脱落的主要蛋白酶。方法:采用慢病毒系统构建稳定表达CD16b的HEK293细胞系。用ADAM10或ADAM17过表达,用ADAM10或ADAM17短发夹RNA抑制,分别用ADAM10或ADAM17重组。每次处理后,用离子霉素或12-肉豆蔻酸酯- 13-乙酸酯(PMA)刺激细胞系12小时。采用免疫沉淀法和免疫印迹法检测细胞膜释放的可溶性CD16b。然后定量比较刺激后细胞上清中可溶性CD16b的含量。结果:成功建立了稳定表达CD16b的HEK293细胞系。当ADAM10过表达CD16b时,离子霉素刺激后CD16b的脱落增加,而PMA刺激后CD16b的脱落没有增加;当ADAM17过表达时,PMA刺激后CD16b的脱落增加,而离子霉素刺激后CD16b的脱落没有增加。同样,当ADAM10被短发夹RNA抑制时,离子霉素刺激后CD16b的脱落减少;当ADAM17被短发夹RNA抑制时,PMA刺激后CD16b的脱落减少。用ADAM10重组并离子霉素刺激表达CD16b的细胞株或用ADAM17重组并PMA刺激表达CD16b的细胞株,CD16b的脱落量再次增加。结论:ADAM10和ADAM17都可以脱除CD16b,但它们具有不同的偏好。ADAM10是离子霉素刺激下的主要分泌酶,ADAM17是PMA刺激下的主要分泌酶。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Role of ADAM10 and ADAM17 in CD16b shedding mediated by different stimulators.

Objective: To investigate the main proteinases responsible for CD16b shedding under different stimulators.

Methods: HEK293 cell line stably expressing CD16b was constructed by lentivirus system. The cell line was then overexpressed with a disintegrin and metalloproteinase 10 (ADAM10) or ADAM17, suppressed with short hairpin RNA of ADAM10 or ADAM17, and reconstituted with ADAM10 or ADAM17, respectively. After each treatment, the cell line was stimulated with ionomycin or phorbol 12-myristate- 13-acetate (PMA) for 12 hours. The soluble CD16b released from cell membrane was detected by immunoprecipition and immunoblot. Quantitation was then implemented to compare the amount of soluble CD16b in cell supernatant after stimulation.

Results: HEK293 cell line stably expressing CD16b was successfully established. When CD16b expressing cell line was overexpressed with ADAM10, shedding of CD16b was increased after stimulation with ionomycin but not PMA; when the cell line overexpressed with ADAM17, shedding of CD16b was increased after stimulation with PMA but not ionomycin. Similarly, when ADAM10 was suppressed by short hairpin RNA, CD16b shedding was decreased after stimulation with ionomycin; when ADAM17 was suppressed by short hairpin RNA, CD16b shedding was decreased after stimulation with PMA. The shedding of CD16b was increased again when CD16b expressing cell line was reconstituted with ADAM10 and stimulated by ionomycin or reconstituted with ADAM17 and stimulated by PMA.

Conclusions: Both ADAM10 and ADAM17 could shed CD16b, but they possess differed preferences. ADAM10 is the main sheddase under stimulation of ionomycin, while ADAM17 is the main sheddase under stimulation of PMA.

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