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Inactivation and proteolytic degradation of perforin within lytic granules upon neutralization of acidic pH.

机译:中和酸性pH后穿孔颗粒中穿孔素的失活和蛋白水解降解。

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摘要

In our recent studies, an inhibitor of vacuolar-type H(+)-ATPase, concanamycin A (CMA) has been shown to neutralize acidic pH in vacuolar organelles, including lytic granules, and to decrease the perforin content markedly. In the present paper, we have further investigated the role of acidification in perforin storage by using CMA. In CD8+ cytotoxic T-lymphocyte (CTL) clones, the amount of perforin decreased rapidly at 30-90 min but no more decrease occurred at 90-120 min after the addition of CMA. Since exposure to actinomycin D, cycloheximide, or brefeldin A failed to reduce the perforin content, the perforin decrease in CMA-treated cells seems to be largely due to a reduction in the perforin already stored in lytic granules, rather than to the inhibition of the de novo synthesis or the intracellular glycoprotein transport of perforin. Diisopropylfluorophosphoridate (DFP) markedly antagonized the decrease in the perforin content in CMA-treated cells, while other protease inhibitors, i.e. antipain, E-64, leupeptin, pepstatin A and phenylmethylsulphonyl fluoride, did not. Nevertheless, DFP hardly reversed the abrogation of the killing activity by CMA. Indeed, the lytic granules prepared from DFP plus CMA-treated cells showed only a marginal level of haemolytic activity. In cell-free experiments using perforin-enriched granule fractions, acidic pH completely blocked the perforin activity. Under the acidic conditions, perforin was more resistant to an inactivation by calcium when exposed to calcium prior to the haemolysis test. Thus, these data suggest that perforin is primarily inactivated, possibly in a calcium-dependent manner, and is subsequently hydrolysed by DFP-sensitive proteases in the lytic granules at neutral pH. We conclude that acidic pH plays an essential role to maintain the integrity of perforin within the lytic granules.
机译:在我们最近的研究中,液泡型H(+)-ATPase抑制剂伴刀豆球蛋白A(CMA)已被证明可中和液泡细胞器(包括溶解颗粒)中的酸性pH,并显着降低穿孔素的含量。在本文中,我们通过使用CMA进一步研究了酸化在穿孔素存储中的作用。在CD8 +细胞毒性T淋巴细胞(CTL)克隆中,添加CMA后,穿孔素的量在30-90分钟时迅速减少,但在90-120分钟时不再减少。由于暴露于放线菌素D,环己酰亚胺或布雷菲德菌素A未能降低穿孔素的含量,因此经CMA处理的细胞中穿孔素的减少似乎主要是由于已经储存在裂解颗粒中的穿孔素的减少,而不是抑制了从头合成或穿孔蛋白的细胞内糖蛋白转运。氟代磷酸二异丙酯(DFP)明显拮抗了CMA处理的细胞中穿孔素含量的降低,而其他蛋白酶抑制剂,即抗痛药,E-64,亮肽素,胃抑素A和苯甲基磺酰氟则没有。尽管如此,DFP几乎无法逆转CMA消除杀伤活性的行为。实际上,由DFP加CMA处理的细胞制备的裂解颗粒仅显示出少量的溶血活性。在使用富含穿孔素的颗粒级分进行的无细胞实验中,酸性pH完全阻断了穿孔素的活性。在酸性条件下,在溶血试验之前,穿孔素暴露于钙时,对钙的失活具有更强的抵抗力。因此,这些数据表明穿孔素主要是失活的,可能是钙依赖性的,随后在中性pH下被溶解颗粒中的DFP敏感性蛋白酶水解。我们得出结论,酸性pH值在维持溶菌颗粒内穿孔素的完整性方面起着至关重要的作用。

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