Open AccessAnalysis of Low Molecular Weight Proteome fromH. pyloriCell Extract Using the High Performance Liquid Chromatography
Author(s) -
JungWon Park,
Kyung Ja Lee,
Kyungmi Kim,
Jung Soo Joo,
Yung Chul Kwon,
HeeShang Youn,
Jae Young Song,
Hyung Lyun Kang,
Kon Ho Lee,
Seung Chul Baik,
WooKon Lee,
Myung Je Cho,
Kwang Ho Rhee
Publication year - 2010
Publication title -
journal of bacteriology and virology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.179
H-Index - 12
eISSN - 2093-0429
pISSN - 1598-2467
DOI - 10.4167/jbv.2010.40.2.67
Subject(s) - polyacrylamide gel electrophoresis , thioredoxin , coomassie brilliant blue , proteome , molecular mass , chromatography , gel electrophoresis , biology , microbiology and biotechnology , proteomics , electroblotting , biochemistry , chemistry , gene , enzyme , staining , genetics
Low molecular proteins (LMPs) which are smaller than 20 kDa are difficult to visible on a standard two-dimensional SDS-polyacrylamide gel electrophoresis (2-D SDS-PAGE) map. LMPs must be enriched appropriately to be analyzed. We isolated LMPs of Helicobacter pylori 26695 from 1-D polyacrylamide gel and digested by pepsin. Pepsin-digested LMPs were separated by HPLC and each fraction was analyzed by hybrid tandem mass spectrometer. Seventy nine peptides, representing 27 genes, including copper ion binding protein (CopP, 7 kDa), thioredoxin (TrxA, 11.9 kDa) and ribosomal protein L23 (Rpl23, 10.5 kDa) were identified. Some proteins larger than 40 kDa including Omp2, Omp21, Omp27, Omp30, Omp32, catalase and HP1083 were also identified. This work may give researchers a useful way to analyse the expressed LMPs which could not be identified on the conventional 2-D SDS-PAGE.
Accelerating Research
Robert Robinson Avenue,
Oxford Science Park, Oxford
OX4 4GP, United Kingdom
Address
John Eccles HouseRobert Robinson Avenue,
Oxford Science Park, Oxford
OX4 4GP, United Kingdom