Literature DB >> 9705494

Non-stoichiometric reduced complexity probes for cDNA arrays.

T Trenkle1, J Welsh, B Jung, F Mathieu-Daude, M McClelland.   

Abstract

A method is presented in which the reduced complexity and non-stoichiometric amplification intrinsic to RNA arbitrarily primed PCR fingerprinting (RAP-PCR) is used to advantage to generate probes for differential screening of cDNA arrays. RAP-PCR fingerprints were converted to probes for human cDNA clones arrayed as Escherichia coli colonies on nylon membranes. Each array contained 18 432 cDNA clones from the IMAGE consortium. Hybridization to approximately 1000 cDNA clones was detected using each RAP-PCR probe. Different RAP-PCR fingerprints gave hybridization patterns having very little overlap (<3%) with each other or with hybridization patterns from total cDNA probes. Consequently, repeated application of RAP-PCR probes allows a greater fraction of the message population to be screened on this type of array than can be achieved with a radiolabeled total cDNA probe. This method was applied to RNA from HaCaT keratinocytes treated with epidermal growth factor. Two RAP-PCR probes detected hybridization to 2000 clones, from which 22 candidate differentially expressed genes were observed. Differential expression was tested for 15 of these clones using RT-PCR and 13 were confirmed. The use of this cDNA array to analyze RAP-PCR fingerprints allowed for an increase in detection of 10-20-fold over the conventional denaturing polyacrylamide gel approach to RAP-PCR or differential display. Throughput is vastly improved by the reduction in cloning and sequencing afforded by the use of arrays. Also, repeated cloning and sequencing of the same gene or of genes already known to be regulated in the system of interest is minimized. The procedure we describe uses inexpensive arrays of plasmid clones spotted as E.coli colonies to detect differential expression, but these reduced complexity probes should also prove useful on arrays of PCR-amplified fragments and on oligonucleotide chips. Genesobserved in this manuscript: H11520, U35048, R48633, H28735, M13918, H12999, H05639, X79781, M31627, H23972, AB000712, R75916, U66894, AF067817.

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Year:  1998        PMID: 9705494      PMCID: PMC147802          DOI: 10.1093/nar/26.17.3883

Source DB:  PubMed          Journal:  Nucleic Acids Res        ISSN: 0305-1048            Impact factor:   16.971


  27 in total

1.  Arbitrarily primed PCR fingerprinting of RNA.

Authors:  J Welsh; K Chada; S S Dalal; R Cheng; D Ralph; M McClelland
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Authors:  P Liang; A B Pardee
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3.  GeneUp: a program to select short PCR primer pairs that occur in multiple members of sequence lists.

Authors:  G Pesole; S Liuni; G Grillo; P Belichard; T Trenkle; J Welsh; M McClelland
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4.  Differential screening of a subtracted cDNA library: a method to search for genes preferentially expressed in multiple tissues.

Authors:  H Jin; X Cheng; L Diatchenko; P D Siebert; C C Huang
Journal:  Biotechniques       Date:  1997-12       Impact factor: 1.993

Review 5.  DNA chips: an array of possibilities.

Authors:  A Marshall; J Hodgson
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6.  Differentially expressed genes in the Trypanosoma brucei life cycle identified by RNA fingerprinting.

Authors:  F Mathieu-Daudé; J Welsh; C Davis; M McClelland
Journal:  Mol Biochem Parasitol       Date:  1998-04-01       Impact factor: 1.759

7.  An efficient approach for the selective isolation of specific transcripts from complex brain mRNA populations.

Authors:  T A Rhyner; N F Biguet; S Berrard; A A Borbély; J Mallet
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Authors:  J Welsh; M McClelland
Journal:  Nucleic Acids Res       Date:  1990-12-25       Impact factor: 16.971

9.  A new approach to high sensitivity differential hybridization.

Authors:  W Boll; J Fujisawa; J Niemi; C Weissmann
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10.  vav, a novel human oncogene derived from a locus ubiquitously expressed in hematopoietic cells.

Authors:  S Katzav; D Martin-Zanca; M Barbacid
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  10 in total

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4.  Detection of differentially expressed genes in an isogenic breast metastasis model using RNA arbitrarily primed-polymerase chain reaction coupled with array hybridization (RAP-array).

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5.  Enhanced microarray performance using low complexity representations of the transcriptome.

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Review 7.  Applications of microarray technology in breast cancer research.

Authors:  C S Cooper
Journal:  Breast Cancer Res       Date:  2001-03-20       Impact factor: 6.466

8.  Overexpression of TSC-22 (transforming growth factor- β-stimulated clone-22) causes marked obesity, splenic abnormality and B cell lymphoma in transgenic mice.

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9.  Vav2 is required for cell spreading.

Authors:  P A Marignani; C L Carpenter
Journal:  J Cell Biol       Date:  2001-07-09       Impact factor: 10.539

10.  Assessment of gene expression in many samples using vertical arrays.

Authors:  Rosa Ana Risques; Gaelle Rondeau; Martin Judex; Michael McClelland; John Welsh
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  10 in total

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