The high percentage of false positives generated by differential display (as

high as 85%) has previously limited the potential of the method. This report describes

an efficient methodology that enables false positives to be discarded prior to cloning, via

reverse Northern analysis. This first step of the screening also allows the detection of

putative lowabundance differential clones. Following cloning, a second reverseNorthern

combined with partial DNA sequencing and RT-PCR detection allows isolation of all

differential cDNAs including very lowabundance clones. Use of the sequential screening

procedure described here led to the isolation of novel tomato genes responding to the

plant hormone ethylene while minimising labor and materials input

Bouquin, Thomas

Bouzayen, Mondher

Jones, Brian

Latché, Alain

Marty, Christel

Pech, Jean-Claude

Zegzouti, Hicham

English

International audienceThe high percentage of false positives generated by differential display (as high as 85%) has previously limited the potential of the method. This report describes an efficient methodology that enables false positives to be discarded prior to cloning, via reverse Northern analysis. This first step of the screening also allows the detection of putative low abundance differential clones. Following cloning, a second reverse Northern combined with partial DNA sequencing and RT-PCR detection allows isolation of all differential cDNAs including very low abundance clones. Use of the sequential screening procedure described here led to the isolation of novel tomato genes responding to the plant hormone ethylene while minimising labor and materials input

HAL: Hyper Article en Ligne

Improved Screening of cDNAs Generated by mRNA Differential Display Enables the Selection of True Positives and the Isolation of Weakly Expressed Messages

Hal-Diderot

The high percentage of false positives generated by differential display (as high as 85%) has previously limited the potential of the method. This report describes an efficient methodology that enables false positives to be discarded prior to cloning, via reverse Northern analysis. This first step of the screening also allows the detection of putative low abundance differential clones. Following cloning, a second reverse Northern combined with partial DNA sequencing and RT-PCR detection allows isolation of all differential cDNAs including very low abundance clones. Use of the sequential screening procedure described here led to the isolation of novel tomato genes responding to the plant hormone ethylene while minimising labor and materials input

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Antisense gene that inhibits synthesis of the hormone ethylene in transgenic plants.

B a u e r

Current protocols in molecular biology.

Differential display of eukaryotic messenger RNA by means of the polymerase chain reaction.

Differentialscreeningof gene expression difference enriched by differential display.

Distribution and cloning of eukaryotic mRNAs by means of differential display: reﬁnements and optimization. Nucleic Acids Res.

Improvements to the differential display method for gene analysis.

Rapid method for screening and cloning cDNA generated in differential mRNA display: application of Northern blot for afﬁnity capturing of cDNA. Nucleic Acids Res.

Rapid selection and classiﬁcation of positive clones generated by mRNA differential display. Nucleic Acids Res.

Structure and expression of three genes encoding ACC oxidase homologs from melon (Cucumis

HAL Université de Toulouse, et Toulouse INP

Improved Screening of cDNAs Generated by mRNA

Differential Display Enables the Selection of True

Positives and the Isolation of Weakly Expressed

Messages

Improved Screening of cDNAs Generated by mRNA Differential Display Enables the Selection of True Positives and the Isolation of Weakly Expressed Messages

Abstract

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Hal-Diderot

Open Archive Toulouse Archive Ouverte

HAL Université de Toulouse, et Toulouse INP