Zhu, Baoli and Smith, Judith A and Tracey, Simon M and Konfortov, Bernard A and Welzel, Katrin and Schalkwyk, Leonard C and Lehrach, Hans and Kollers, Sonja and Masabanda, Julio and Buitkamp, Johannes and Fries, Ruedi and Williams, John L and Miller, J Ross (1999) A 5× genome coverage bovine BAC library: production, characterization, and distribution. Mammalian Genome, 10 (7). pp. 706-709. DOI https://doi.org/10.1007/s003359901075
Zhu, Baoli and Smith, Judith A and Tracey, Simon M and Konfortov, Bernard A and Welzel, Katrin and Schalkwyk, Leonard C and Lehrach, Hans and Kollers, Sonja and Masabanda, Julio and Buitkamp, Johannes and Fries, Ruedi and Williams, John L and Miller, J Ross (1999) A 5× genome coverage bovine BAC library: production, characterization, and distribution. Mammalian Genome, 10 (7). pp. 706-709. DOI https://doi.org/10.1007/s003359901075
Zhu, Baoli and Smith, Judith A and Tracey, Simon M and Konfortov, Bernard A and Welzel, Katrin and Schalkwyk, Leonard C and Lehrach, Hans and Kollers, Sonja and Masabanda, Julio and Buitkamp, Johannes and Fries, Ruedi and Williams, John L and Miller, J Ross (1999) A 5× genome coverage bovine BAC library: production, characterization, and distribution. Mammalian Genome, 10 (7). pp. 706-709. DOI https://doi.org/10.1007/s003359901075
Abstract
A bovine large-insert DNA library has been constructed in a Bacterial Artificial Chromosome (BAC) vector. The source DNA was derived from lymphocytes of a Jersey male. High-molecular-weight DNA fragments were produced by treatment with EcoRI/EcoRI methylase and cloned into the EcoRI site of pBACe3.6. In total, 157,240 individual BACs have been picked into 384-well plates. Approximately 190 randomly chosen clones have been characterized by Pulsed Field Gel Electrophoresis (PFGE) and have an average insert size of 105 kb, suggesting library coverage representing 5-6 genome equivalents. The frequency of clones without inserts is 4%. The chromosomal location of 51 BACs was studied by FISH; 3 showed more than one signal, indicating a chimerism frequency of roughly 6%. Approximately 50% of the clones in the library contain Simple Repeat Sequences (microsatellites), and 4% of the clones contain centromeric repeats. Insert stability was assessed by restriction digestion of DNA prepared from 20 clones after serial culture for one and three nights. Only one clone showed any evidence of an altered restriction pattern. Clones from 360 x 384-well plates (138,240 colonies) were gridded onto high-density membranes, and PCR superpools were produced from the same set of clones. Both membranes and superpools are available from the RZPD, Berlin (http://www.rzpd.de). PCR 4-D superpools have been prepared from an additional 23,000 clones. The library has been screened for a total of 24 single-copy sequences; positive clones have been obtained in all cases.
Item Type: | Article |
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Uncontrolled Keywords: | Chromosomes; Animals; Chimera; Cattle; Bacteria; DNA Primers; Cloning, Molecular; Base Sequence; Microsatellite Repeats; Genomic Library; Genetic Vectors; Male |
Subjects: | Q Science > QH Natural history > QH426 Genetics |
Divisions: | Faculty of Science and Health Faculty of Science and Health > Life Sciences, School of |
SWORD Depositor: | Unnamed user with email elements@essex.ac.uk |
Depositing User: | Unnamed user with email elements@essex.ac.uk |
Date Deposited: | 23 Oct 2014 11:27 |
Last Modified: | 04 Dec 2024 06:47 |
URI: | http://repository.essex.ac.uk/id/eprint/11125 |