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基质辅助激光解吸/电离-四极杆离子阱-飞行时间质谱测序解析了通过对人血浆蛋白质组中触珠蛋白衍生物进行胶内胰蛋白酶消化获得的未知肽段的结构。

Matrix-assisted laser desorption/ionization- quadrupole ion trap-time of flight mass spectrometry sequencing resolves structures of unidentified peptides obtained by in-gel tryptic digestion of haptoglobin derivatives from human plasma proteomes.

作者信息

Koy Cornelia, Mikkat Stefan, Raptakis Emmanuel, Sutton Chris, Resch Martin, Tanaka Koichi, Glocker Michael O

机构信息

Proteome Center Rostock, University of Rostock, Rostock, Germany.

出版信息

Proteomics. 2003 Jun;3(6):851-8. doi: 10.1002/pmic.200300381.

DOI:10.1002/pmic.200300381
PMID:12833508
Abstract

Two-dimensional gel electrophoresis-separated and excised haptoglobin alpha2-chain protein spots were subjected to in-gel digestion with trypsin. Previously unassigned peptide ion signals observed in mass spectrometric fingerprinting experiments were sequenced using the matrix-assisted laser desorption/ionization-quadrupole ion trap-time of flight (MALDI-QIT-TOF) mass spectrometer and showed that the haptoglobin alpha-chain derivative under study was cleaved by trypsin unspecifically. Abundant cleavages occurred C-terminal to histidine residues at H23, H28, and H87. In addition, mild acidic hydrolysis leading to cleavage after aspartic acid residues at D13 was observed. The uninterpreted tandem mass spectrometry (MS/MS) spectrum of the peptide with ion signal at 2620.19 was submitted to database search and yielded the identification of the corresponding peptide sequence comprising amino acids (aa) aa65-87 from the haptoglobin alpha-chain protein. Also, the presence of a mixture of two tryptic peptides (mass to charge ratio m/z 1708.8; aa40-54, and aa99-113, respectively), that is caused by a tiny sequence variation between the two repeats in the haptoglobin alpha2-chain protein was resolved by MS/MS fragmentation using the MALDI-QIT-TOF mass spectrometer instrument. Advantageous features such as (i) easy parent ion creation, (ii) minimal sample consumption, and (iii) real collision induced dissociation conditions, were combined successfully to determine the amino acid sequences of the previously unassigned peptides. Hence, the novel mass spectrometric sequencing method applied here has proven effective for identification of distinct molecular protein structures.

摘要

将二维凝胶电泳分离并切除的触珠蛋白α2链蛋白斑点用胰蛋白酶进行胶内消化。在质谱指纹图谱实验中观察到的先前未归属的肽离子信号,使用基质辅助激光解吸/电离-四极杆离子阱-飞行时间(MALDI-QIT-TOF)质谱仪进行测序,结果表明所研究的触珠蛋白α链衍生物被胰蛋白酶非特异性切割。在H23、H28和H87的组氨酸残基的C末端发生了大量切割。此外,还观察到温和的酸性水解导致D13处天冬氨酸残基后的切割。将离子信号在2620.19处的肽的未解释串联质谱(MS/MS)谱提交给数据库搜索,鉴定出了来自触珠蛋白α链蛋白的相应肽序列,其包含氨基酸(aa)aa65-87。同样,通过使用MALDI-QIT-TOF质谱仪进行MS/MS碎片化,解析了触珠蛋白α2链蛋白中两个重复序列之间微小序列差异导致的两种胰蛋白酶肽(质荷比m/z 1708.8;分别为aa40-54和aa99-113)混合物的存在。诸如(i)易于产生母离子、(ii)样品消耗极少以及(iii)真实的碰撞诱导解离条件等有利特征成功结合,以确定先前未归属肽的氨基酸序列。因此,这里应用的新型质谱测序方法已被证明对于鉴定不同的分子蛋白结构是有效的。

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