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从嗜铬细胞瘤中提取的嗜铬粒蛋白B片段368 - 417被磷酸化的证据。

Evidence that the chromogranin B fragment 368-417 extracted from a pheochromocytoma is phosphorylated.

作者信息

Dahma H, Gourlet P, Vandermeers A, Vandermeers-Piret M C, Robberecht P

机构信息

Department of Biochemistry and Nutrition, Medical School, Université Libre de Bruxelles, B-1070, Brussels, Belgium.

出版信息

Peptides. 2001 Sep;22(9):1491-9. doi: 10.1016/s0196-9781(01)00471-5.

Abstract

A rabbit antiserum was raised against a synthetic peptide corresponding to residues 403 to 417 of human chromogranin B. This peptide was chosen to match the potential C-terminal end of a putative proteolytic fragment of the protein located between dibasic doublets in positions 366-367 and in positions 418-419 of the precursor. A radioimmunoassay based on this antiserum was developed and used to detect the protein or a fragment thereof in a pheochromocytoma tumor extract. One fragment was purified to homogeneity by successive reverse-phase HPLC chromatographies. The N-terminal sequence established by automated Edman degradation, was N-Y-P-S-L-E-L-D-K-M-A-H-G-Y-G-E-E-S-E-E-E-R corresponding to the 368-389 sequence of human chromogranin B. Taking into account the specificity of the antiserum used for peptide identification and alignment with the precursor sequence, we deduced that the purified peptide was chromogranin B (368-417) and represented a new peptide generated by limited proteolysis of chromogranin B. Combining electrospray mass-spectrometry and enzymatic dephosphorylation, we demonstrated that this peptide was phosphorylated.

摘要

制备了一种兔抗血清,其针对的是与人类嗜铬粒蛋白B的403至417位残基相对应的合成肽。选择该肽是为了匹配该蛋白质假定蛋白水解片段的潜在C末端,该片段位于前体的366 - 367位和418 - 419位的双碱性双峰之间。基于该抗血清开发了一种放射免疫测定法,并用于检测嗜铬细胞瘤肿瘤提取物中的该蛋白质或其片段。通过连续的反相高效液相色谱法将一个片段纯化至同质。通过自动Edman降解确定的N末端序列为N - Y - P - S - L - E - L - D - K - M - A - H - G - Y - G - E - E - S - E - E - E - R,对应于人类嗜铬粒蛋白B的368 - 389序列。考虑到用于肽鉴定的抗血清的特异性以及与前体序列的比对,我们推断纯化的肽是嗜铬粒蛋白B(368 - 417),并且代表了由嗜铬粒蛋白B的有限蛋白水解产生的一种新肽。结合电喷雾质谱法和酶促去磷酸化,我们证明了该肽是磷酸化的。

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