Comparison of the unlabeled and labeled pre-mRNA splicing assays in vitro  

作　　者：TIAN XU BU JING XIN HONG ZHI YAO JIE YANG 

机构地区：[1]Department of Immunology, Tianjin Medical University, Tianjin, P. R. China [2]Clinical Biochemistry Lab, the General Hospital of Tianfin Medical University, Tianfin , P . R . China

出　　处：《Journal of Microbiology and Immunology》2006年第4期313-317,共5页中华微生物学和免疫学（英文版）

基　　金：We thank Hao Zhang for technical assistance, Dr. Robin Reed for providing AdML plasmids. The work was supported by grants from National Natural Science Foundation of China （30670441, 30300070）;Program for New Century Excellent Talents in University （NCET-04-0245）; Specialized Fund for the Doctoral Program of Higher Education （20040062003）;Tianjin Municipal Science and Technology Commission （043802811）.

摘　　要：Pre-mRNA splicing is a fundamental process required for the expression of most metazoan genes. It is carried out by the spliceosome that catalyzes the removal of non-coding intron sequences to ligate exons into mature mRNA prior to transport and translation. The purpose of our study is to explore whether the in vitro unlabeled pre-mRNA splicing assay could be performed as an alternative method of splicing reaction other than the radiolabeled one. Two different splicing methods in vitro, 32p labeled and unlabeled pre-mRNA as the substrates in the reaction, were investigated. The radiolabeled products were visualized by autoradiography while the unlabeled products were observed by Ethidium Bromide （EB） staining. As a result, although there are more unspecific bands in the EB staining assay than 32p labeled one, the RNA products of in vitro splicing could be observed clearly. This suggests that the unlabeled pre-mRNA splicing assay can be an optional substitution for the isotope-labeled assay.Pre-mRNA splicing is a fundamental process required for the expression of most metazoan genes. It is carried out by the spliceosome that catalyzes the removal of non-coding intron sequences to ligate exons into mature mRNA prior to transport and translation. The purpose of our study is to explore whether the in vitro unlabeled pre-mRNA splicing assay could be performed as an alternative method of splicing reaction other than the radiolabeled one. Two different splicing methods in vitro , P labeled and unlabeled pre-mRNA as the substrates in the reaction, were investigated. The radiolabeled products were visualized by autoradiography while the unlabeled products were observed by Ethidium Bromide (EB) staining. As a result, although there are more unspecific bands in the EB staining assay than 32P labeled one, the RNA products of in vitro splicing could be observed clearly. This suggests that the unlabeled pre-mRNA splicing assay can be an optional substitution for the isotope-labeled assay.

关 键 词：Pre-mRNA splicing Spliceoseme Ethidiurn Bromide staining Autoradiography 

分 类 号：Q78[生物学—分子生物学]