Analysis of mRNA with microsomal fractionation using a SAGE-based DNA microarray system facilitates identification of the genes encoding secretory proteins

Nobuaki Toyoda; Shigenori Nagai; Yuya Terashima; Kazushi Motomura; Makoto Haino; Shin-ichi Hashimoto; Hajime Takizawa; Kouji Matsushima

doi:10.1101/gr.709603

Analysis of mRNA with microsomal fractionation using a SAGE-based DNA microarray system facilitates identification of the genes encoding secretory proteins

Genome Res. 2003 Jul;13(7):1728-36. doi: 10.1101/gr.709603. Epub 2003 Jun 12.

Authors

Nobuaki Toyoda¹, Shigenori Nagai, Yuya Terashima, Kazushi Motomura, Makoto Haino, Shin-ichi Hashimoto, Hajime Takizawa, Kouji Matsushima

Affiliation

¹ Department of Molecular Preventive Medicine & SORST, School of Medicine, The University of Tokyo, Bunkyo-ku, Tokyo 113-0033, Japan.

Abstract

In the regulation of host defense responses such as inflammation and immunity, the secretory proteins, including membrane proteins, play central roles. Although many secretory proteins have been identified by using methods such as differential display, random screening, or the signal sequence trap method, each method suffers from poor reproducibility, low sensitivity, or time-consuming or laborious work. Therefore, the strategy for facilitating the selection of the genes encoding the secretory proteins is desired. In this paper, we describe a system for isolating the genes encoding secretory proteins by analyzing mRNAs with microsomal fractionation on serial analysis of gene expression (SAGE)-based DNA microarray system. This system succeeded in discriminating the genes encoding secretory proteins from ones encoding nonsecretory proteins with 80% accuracy. We applied this system to human T lymphocytes. As a result, we were able to identify the genes that are not only encoding secretory proteins but also expressing selectively in a specific subset of T lymphocytes. The SAGE-based DNA microarray system is a promising system to identify the genes encoding specific secretory proteins.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Amino Acid Sequence
CD4-Positive T-Lymphocytes / chemistry
CD4-Positive T-Lymphocytes / cytology
CD4-Positive T-Lymphocytes / metabolism
Cell Line
Cloning, Molecular / methods
DNA, Complementary / analysis
Gene Expression Profiling / methods*
Genes / genetics
Green Fluorescent Proteins
Humans
Kidney / chemistry
Kidney / cytology
Kidney / embryology
Kidney / metabolism
Luminescent Proteins / biosynthesis
Luminescent Proteins / genetics
Lymphocyte Activation / genetics
Membrane Proteins / biosynthesis
Membrane Proteins / genetics*
Microsomes / chemistry*
Microsomes / metabolism*
Molecular Sequence Data
Oligonucleotide Array Sequence Analysis / methods*
Polyribosomes / chemistry
Polyribosomes / genetics
Protein Biosynthesis / genetics
Proteins / genetics*
Proteins / metabolism*
RNA, Messenger / analysis*
Recombinant Proteins / biosynthesis
Recombinant Proteins / genetics
Sequence Analysis, RNA / methods
Subcellular Fractions / chemistry
Subcellular Fractions / metabolism
T-Lymphocyte Subsets / chemistry
T-Lymphocyte Subsets / cytology
T-Lymphocyte Subsets / metabolism
Th1 Cells / chemistry
Th1 Cells / cytology
Th1 Cells / metabolism
Th2 Cells / chemistry
Th2 Cells / cytology
Th2 Cells / metabolism

Substances

DNA, Complementary
Luminescent Proteins
Membrane Proteins
Proteins
RNA, Messenger
Recombinant Proteins
Green Fluorescent Proteins