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大鼠催乳素的22K变体:与催乳素-(1-173)相同、储存于分泌颗粒及受调控释放的证据。

The 22K variant of rat prolactin: evidence for identity to prolactin-(1-173), storage in secretory granules, and regulated release.

作者信息

Anthony P K, Stoltz R A, Pucci M L, Powers C A

机构信息

Department of Pharmacology, New York Medical College, Valhalla 10595.

出版信息

Endocrinology. 1993 Feb;132(2):806-14. doi: 10.1210/endo.132.2.8425495.

Abstract

Western blot analyses of the rat pituitary have detected a 22K PRL variant distinct from intact PRL (25K). We recently reported that glandular kallikrein (GK), an estrogen-induced lactotroph protease, can process PRL in vitro from a 25K form to a 22K form in a thiol-dependent cleavage at Arg174-Arg175 to remove 23 amino acids. We also detected an estrogen- and thiol-induced 22K PRL variant in the rat pituitary comigrating with a PRL product generated by in vitro processing with GK and carboxypeptidase-B. This study addressed whether the in vivo 22K PRL variant originates through a GK-like cleavage and is a regulated secretory product of the rat pituitary. A polyclonal antipeptide antiserum was raised against a synthetic peptide [PRL-(163-173)] representing the new C-terminus after GK and carboxypeptidase-B processing. In slot and Western blots, this antiserum (CT-antiserum) specifically recognized PRL processed in vitro by GK and carboxypeptidase-B and did not recognize intact PRL or PRL cleaved by GK alone. Western blot analysis of rat pituitary extracts with CT-antiserum specifically detected an estrogen- and thiol-induced 22K band that comigrated with a PRL product generated by in vitro processing with GK and carboxypeptidase-B. This 22K band was concentrated in subcellular fractions of the pituitary enriched in secretory granules. During short term incubations in medium 199, pituitaries from normal adult female rats released substantial amounts of 22K PRL; in contrast, male pituitaries did not release detectable 22K PRL. The release of 22K PRL from female pituitaries was powerfully blocked by bromocriptine, a dopaminergic agonist. GK was also released from pituitaries of female, but not male, rats, and GK release was inhibited by bromocriptine. The results identify the 22K PRL variant as PRL-(1-173), which is consistent with GK-like processing at Arg174-Arg175, followed by carboxypeptidase-B-like processing. The results also show that 22K PRL is a natural female-specific secretory product of the rat pituitary under inhibitory dopaminergic control.

摘要

对大鼠垂体进行的蛋白质免疫印迹分析检测到一种与完整催乳素(25K)不同的22K催乳素变体。我们最近报道,腺激肽释放酶(GK)是一种雌激素诱导的催乳细胞蛋白酶,它可以在体外将催乳素从25K形式加工成22K形式,在Arg174 - Arg175处进行硫醇依赖性切割,去除23个氨基酸。我们还在大鼠垂体中检测到一种雌激素和硫醇诱导的22K催乳素变体,它与用GK和羧肽酶B进行体外加工产生的催乳素产物迁移率相同。本研究探讨了体内22K催乳素变体是否通过类似GK的切割产生,以及它是否是大鼠垂体的一种受调节的分泌产物。针对代表GK和羧肽酶B加工后的新C末端的合成肽[催乳素 - (163 - 173)]制备了多克隆抗肽抗血清。在狭缝印迹和蛋白质免疫印迹中,这种抗血清(CT抗血清)特异性识别由GK和羧肽酶B在体外加工的催乳素,而不识别完整的催乳素或仅由GK切割的催乳素。用CT抗血清对大鼠垂体提取物进行蛋白质免疫印迹分析,特异性检测到一条雌激素和硫醇诱导的22K条带,它与用GK和羧肽酶B进行体外加工产生的催乳素产物迁移率相同。这条22K条带集中在垂体中富含分泌颗粒的亚细胞组分中。在199培养基中短期孵育期间,正常成年雌性大鼠的垂体释放大量的22K催乳素;相比之下,雄性垂体未释放可检测到的22K催乳素。雌性垂体释放22K催乳素受到多巴胺能激动剂溴隐亭的强烈抑制。GK也从雌性大鼠的垂体中释放,但不从雄性大鼠的垂体中释放,并且GK的释放受到溴隐亭的抑制。结果确定22K催乳素变体为催乳素 - (1 - 173),这与在Arg174 - Arg175处进行类似GK的加工,随后进行类似羧肽酶B的加工一致。结果还表明,22K催乳素是大鼠垂体在多巴胺能抑制控制下的一种天然的雌性特异性分泌产物。

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