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5-叠氮基-8-乙炔基-NADP:一种双功能、点击化学光亲和探针,用于鉴定 NADP 受体。

5-Azido-8-ethynyl-NAADP: A bifunctional, clickable photoaffinity probe for the identification of NAADP receptors.

机构信息

Department of Pharmacology, University of Minnesota Medical School, 312 Church St., Minneapolis, MN 55455-0217, United States of America.

Department of Medicinal and Biological Chemistry, University of Toledo College of Pharmacy and Pharmaceutical Sciences, 3000 Arlington Avenue, Toledo, OH 43614, United States of America.

出版信息

Biochim Biophys Acta Mol Cell Res. 2019 Jul;1866(7):1180-1188. doi: 10.1016/j.bbamcr.2018.11.017. Epub 2018 Dec 4.

DOI:10.1016/j.bbamcr.2018.11.017
PMID:30521871
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8101546/
Abstract

Nicotinic acid adenine dinucleotide phosphate is an evolutionarily conserved second messenger, which mobilizes Ca from acidic stores. The molecular identity of the NAADP receptor has yet to be defined. In pursuit of isolating and identifying NAADP-binding proteins, we synthesized and characterized a bifunctional probe that incorporates both a photoactivatable crosslinking azido moiety at the 5-position of the nicotinic ring and a 'clickable' ethynyl moiety to the 8-adenosyl position in NAADP. Microinjection of this 5N-8-ethynyl-NAADP into cultured U2OS cells induced robust Ca responses. Higher concentrations of 5N-8-ethynyl were required to elicit Ca release or displace P-NAADP in radioligand binding experiments in sea urchin egg homogenates. In human cell extracts, incubation of P-5N-8-ethynyl-NAADP followed by UV irradiation resulted in selective labeling of 23 kDa and 35 kDa proteins and photolabeling of these proteins was prevented when incubated in the presence of unlabeled NAADP. Compared to the monofunctional P-5N-NAADP, the clickable P-5N-8-ethynyl-NAADP demonstrated less labeling of the 23 kDa and 35 kDa proteins (~3-fold) but provided an opportunity for further enrichment through the 'clickable' ethynyl moiety. No proteins were specifically labeled by P-5N-8-ethynyl-NAADP in sea urchin egg homogenate. These experiments demonstrate that 5N-8-ethynyl-NAADP is biologically active and selectively labels putative NAADP-binding proteins in mammalian systems, evidencing a 'bifunctional' probe with utility for isolating NAADP-binding proteins.

摘要

烟酰胺腺嘌呤二核苷酸磷酸是一种进化上保守的第二信使,它从酸性储存库中动员 Ca。NAADP 受体的分子身份尚未确定。为了分离和鉴定 NAADP 结合蛋白,我们合成并表征了一种双功能探针,该探针在烟酰胺环的 5 位包含一个光活化交联叠氮部分,在 NAADP 的 8-腺苷基位置包含一个“点击”乙炔基部分。将这种 5N-8-乙炔基-NAADP 微注射到培养的 U2OS 细胞中会诱导强烈的 Ca 反应。在海胆卵匀浆的放射性配体结合实验中,需要更高浓度的 5N-8-乙炔基才能引发 Ca 释放或置换 P-NAADP。在人细胞提取物中,孵育 P-5N-8-乙炔基-NAADP 后进行 UV 照射导致 23 kDa 和 35 kDa 蛋白的选择性标记,并且当在未标记的 NAADP 存在下孵育时,这些蛋白的光标记被阻止。与单功能 P-5N-NAADP 相比,可点击的 P-5N-8-乙炔基-NAADP 对 23 kDa 和 35 kDa 蛋白的标记较少(约 3 倍),但通过“可点击”乙炔基部分提供了进一步富集的机会。在海胆卵匀浆中,没有蛋白质被 P-5N-8-乙炔基-NAADP 特异性标记。这些实验表明,5N-8-乙炔基-NAADP 具有生物活性,并且选择性地标记哺乳动物系统中的假定 NAADP 结合蛋白,证明了具有分离 NAADP 结合蛋白用途的“双功能”探针。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6450/8101546/6c4b93e287fe/nihms-1674292-f0001.jpg

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