A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNA
<p>Abstract</p> <p>Background</p> <p>The transcribed sequences of a cell, the transcriptome, represent the trans-acting fraction of the genetic information, yet eukaryotic cDNA libraries are typically made from only the poly-adenylated fraction. The non-coding or transl...
| Main Authors: | , , |
|---|---|
| Format: | Article |
| Language: | English |
| Published: |
BMC
2007-10-01
|
| Series: | BMC Genomics |
| Online Access: | http://www.biomedcentral.com/1471-2164/8/363 |
| id |
doaj-cc7ba930b84d47879e67484446501ee9 |
|---|---|
| record_format |
Article |
| spelling |
doaj-cc7ba930b84d47879e67484446501ee92020-11-24T23:17:12ZengBMCBMC Genomics1471-21642007-10-018136310.1186/1471-2164-8-363A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNAGitelman InnaBarvish ZeevDavis Claytus<p>Abstract</p> <p>Background</p> <p>The transcribed sequences of a cell, the transcriptome, represent the trans-acting fraction of the genetic information, yet eukaryotic cDNA libraries are typically made from only the poly-adenylated fraction. The non-coding or translated but non-polyadenylated RNAs are therefore not represented. The goal of this study was to develop a method that would more completely represent the transcriptome in a useful format, avoiding over-representation of some of the abundant, but low-complexity non-translated transcripts.</p> <p>Results</p> <p>We developed a combination of self-subtraction and directional cloning procedures for this purpose. Libraries were prepared from partially degraded (hydrolyzed) total RNA from three different species. A restriction endonuclease site was added to the 3' end during first-strand synthesis using a directional random-priming technique. The abundant non-polyadenylated rRNA and tRNA sequences were largely removed by using self-subtraction to equalize the representation of the various RNA species. Sequencing random clones from the libraries showed that 87% of clones were in the forward orientation with respect to known or predicted transcripts. 70% matched identified or predicted translated RNAs in the sequence databases. Abundant mRNAs were less frequent in the self-subtracted libraries compared to a non-subtracted mRNA library. 3% of the sequences were from known or hypothesized ncRNA loci, including five matches to miRNA loci.</p> <p>Conclusion</p> <p>We describe a simple method for making high-quality, directional, random-primed, cDNA libraries from small amounts of degraded total RNA. This technique is advantageous in situations where a cDNA library with complete but equalized representation of transcribed sequences, whether polyadenylated or not, is desired.</p> http://www.biomedcentral.com/1471-2164/8/363 |
| collection |
DOAJ |
| language |
English |
| format |
Article |
| sources |
DOAJ |
| author |
Gitelman Inna Barvish Zeev Davis Claytus |
| spellingShingle |
Gitelman Inna Barvish Zeev Davis Claytus A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNA BMC Genomics |
| author_facet |
Gitelman Inna Barvish Zeev Davis Claytus |
| author_sort |
Gitelman Inna |
| title |
A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNA |
| title_short |
A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNA |
| title_full |
A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNA |
| title_fullStr |
A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNA |
| title_full_unstemmed |
A method for the construction of equalized directional cDNA libraries from hydrolyzed total RNA |
| title_sort |
method for the construction of equalized directional cdna libraries from hydrolyzed total rna |
| publisher |
BMC |
| series |
BMC Genomics |
| issn |
1471-2164 |
| publishDate |
2007-10-01 |
| description |
<p>Abstract</p> <p>Background</p> <p>The transcribed sequences of a cell, the transcriptome, represent the trans-acting fraction of the genetic information, yet eukaryotic cDNA libraries are typically made from only the poly-adenylated fraction. The non-coding or translated but non-polyadenylated RNAs are therefore not represented. The goal of this study was to develop a method that would more completely represent the transcriptome in a useful format, avoiding over-representation of some of the abundant, but low-complexity non-translated transcripts.</p> <p>Results</p> <p>We developed a combination of self-subtraction and directional cloning procedures for this purpose. Libraries were prepared from partially degraded (hydrolyzed) total RNA from three different species. A restriction endonuclease site was added to the 3' end during first-strand synthesis using a directional random-priming technique. The abundant non-polyadenylated rRNA and tRNA sequences were largely removed by using self-subtraction to equalize the representation of the various RNA species. Sequencing random clones from the libraries showed that 87% of clones were in the forward orientation with respect to known or predicted transcripts. 70% matched identified or predicted translated RNAs in the sequence databases. Abundant mRNAs were less frequent in the self-subtracted libraries compared to a non-subtracted mRNA library. 3% of the sequences were from known or hypothesized ncRNA loci, including five matches to miRNA loci.</p> <p>Conclusion</p> <p>We describe a simple method for making high-quality, directional, random-primed, cDNA libraries from small amounts of degraded total RNA. This technique is advantageous in situations where a cDNA library with complete but equalized representation of transcribed sequences, whether polyadenylated or not, is desired.</p> |
| url |
http://www.biomedcentral.com/1471-2164/8/363 |
| work_keys_str_mv |
AT gitelmaninna amethodfortheconstructionofequalizeddirectionalcdnalibrariesfromhydrolyzedtotalrna AT barvishzeev amethodfortheconstructionofequalizeddirectionalcdnalibrariesfromhydrolyzedtotalrna AT davisclaytus amethodfortheconstructionofequalizeddirectionalcdnalibrariesfromhydrolyzedtotalrna AT gitelmaninna methodfortheconstructionofequalizeddirectionalcdnalibrariesfromhydrolyzedtotalrna AT barvishzeev methodfortheconstructionofequalizeddirectionalcdnalibrariesfromhydrolyzedtotalrna AT davisclaytus methodfortheconstructionofequalizeddirectionalcdnalibrariesfromhydrolyzedtotalrna |
| _version_ |
1725584215196565504 |