Sensitive nonradioactive dot blot/ribonuclease protection assay for quantitative determination of mRNA

被引：20

作者：

Zhan, JH ^{[1
]}

Fahimi, HD ^{[1
]}

Voelkl, A ^{[1
]}

机构：

[1] UNIV HEIDELBERG,DEPT ANAT & CELL BIOL 2,D-69120 HEIDELBERG,GERMANY

来源：

BIOTECHNIQUES | 1997年 / 22卷 / 03期

关键词：

D O I：

10.2144/97223st05

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

We have developed a simple and sensitive method for the rapid quantitation of mRNA from a cell cultures and small tissue samples. The method combines the high sensitivity and specificity of the ribonuclease protection assay with simple handling and rapid execution of dot blotting. The use of digoxygenin-labeled cRNA probes eliminates all problems associated with radioisotopes commonly used in the ribonuclease protection assay. The RNA preparation is dotted directly onto nylon membranes, and after hybridization the filters are treated with ribonuclease A, which remove the nonhybridized single-stranded RNA. The mRNA-hybrid is then visualized by the chemiluminescence technique using labeled anti-diogoxigenin antibody, and the signal intensity is quantitated. Comparison with the Northern blotting ribonuclease protection assay revealed that this dot blot technique is almost ten times more sensitive and that its signals are linear over a wide range of RNA concentrations (0.01-10 mu g/mu L/dot). This method seems particularly valuable for simultaneous processing of large numbers of samples containing a wide range of RNA concentrations.

引用

页码：500 / &

页数：5

共 21 条

[1] DETECTION OF B19-PARVOVIRUS INFECTIONS BY A DOT BLOT HYBRIDIZATION ASSAY USING A DIGOXIGENIN-LABELED PROBE [J].

AZZI, A ;

ZAKRZEWSKA, K ;

GENTILOMI, G ;

MUSIANI, M ;

ZERBINI, M .

JOURNAL OF VIROLOGICAL METHODS, 1990, 27 (02) :125-133

[2] SIZING AND MAPPING OF EARLY ADENOVIRUS MESSENGER-RNAS BY GEL-ELECTROPHORESIS OF S1 ENDONUCLEASE-DIGESTED HYBRIDS [J].

BERK, AJ ;

SHARP, PA .

CELL, 1977, 12 (03) :721-732

[3] SINGLE-STEP METHOD OF RNA ISOLATION BY ACID GUANIDINIUM THIOCYANATE PHENOL CHLOROFORM EXTRACTION [J].

CHOMCZYNSKI, P ;

SACCHI, N .

ANALYTICAL BIOCHEMISTRY, 1987, 162 (01) :156-159

[4] QUANTITATIVE MOLECULAR HYBRIDIZATION WITH UNFRACTIONATED, SOLUBILIZED CELLS USING RNA PROBES AND POLYACRYLAMIDE-GEL ELECTROPHORESIS [J].

FIRESTEIN, GS ;

GARDNER, SM ;

ROEDER, WD .

ANALYTICAL BIOCHEMISTRY, 1987, 167 (02) :381-386

[5] USE OF CRNA DIGOXIGENIN-LABELED PROBES FOR DETECTION OF ENTEROVIRUSES IN HUMANS AND IN THE ENVIRONMENT [J].

FUCHS, F ;

LEPARC, I ;

KOPECKA, H ;

GARIN, D ;

AYMARD, M .

JOURNAL OF VIROLOGICAL METHODS, 1993, 42 (2-3) :217-226

[6] A TOTAL EXTRACT DOT BLOT HYBRIDIZATION PROCEDURE FOR MESSENGER-RNA QUANTITATION IN SMALL SAMPLES OF TISSUES OR CULTURED-CELLS [J].

GRIMES, A ;

MCARDLE, HJ ;

MERCER, JFB .

ANALYTICAL BIOCHEMISTRY, 1988, 172 (02) :436-443

[7]

HAINES DS, 1992, BIOTECHNIQUES, V12, P736

[8] USE OF A DOT BLOT HYBRIDIZATION METHOD FOR IDENTIFICATION OF PURE TRANSFER-RNA SPECIES ON DIFFERENT MEMBRANES [J].

HEITZLER, J ;

MARECHALDROUARD, L ;

DIRHEIMER, G ;

KEITH, G .

BIOCHIMICA ET BIOPHYSICA ACTA, 1992, 1129 (03) :273-277

[9]

HOLTKE HJ, 1992, BIOTECHNIQUES, V12, P104

[10] POSSIBLE ROLE OF VARIANT RNA TRANSCRIPTS IN THE REGULATION OF EPIDERMAL GROWTH-FACTOR RECEPTOR EXPRESSION IN HUMAN PLACENTA [J].

ILEKIS, JV ;

STARK, BC ;

SCOCCIA, B .

MOLECULAR REPRODUCTION AND DEVELOPMENT, 1995, 41 (02) :149-156

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