The use of competitive PCR mimic to evaluate a Limulus lambda phage genomic DNA library

The use of competitive PCR mimic to evaluate a Limulus lambda phage genomic DNA library

1. A lambda phage genomic DNA library for Limulus (L.) polyphemus brain was constructed using the AGEM-12 vector and the host strain KW251. 2. The primary library contained approximately 1.275 x 10(6) independent clones, increasing upon amplfication to 6.66 x 10(9) pfu/ml in a total volume of 58 ml....

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Veröffentlicht in:Cellular and molecular neurobiology 2000-08, Vol.20 (4), p.509-520
Hauptverfasser: Wang, Y, Cao, Z, Reid, E A, Newkirk, R F, Ivy, M T, Townsel, J G
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Sprache:eng
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Animals
Bacteriophage lambda - genetics
Brain Chemistry - genetics
DNA - analysis
DNA libraries
Genomic Library
Horseshoe Crabs - genetics
Horseshoe Crabs - metabolism
Lambda Phage
Limulus polyphemus
Polymerase Chain Reaction
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container_end_page 520
container_issue 4
container_start_page 509
container_title Cellular and molecular neurobiology
container_volume 20
creator Wang, Y
Cao, Z
Reid, E A
Newkirk, R F
Ivy, M T
Townsel, J G
description 1. A lambda phage genomic DNA library for Limulus (L.) polyphemus brain was constructed using the AGEM-12 vector and the host strain KW251. 2. The primary library contained approximately 1.275 x 10(6) independent clones, increasing upon amplfication to 6.66 x 10(9) pfu/ml in a total volume of 58 ml. 3. A total of 28 clones was randomly chosen for a determination of the average size of inserts in the library. All clones contained inserts and the average size was 14.9 kb, ranging from 11.7 to 28.0 kb. The library provides a 10-fold equivalent of the L. polyphemus genome. 4. A new approach for evaluating a genomic DNA library was developed, in which competitive PCR MIMIC was employed to determine the target gene copy number in both constructed library and brain genomic DNA. The putative protein kinase C epsilon (PKCepsilon) was selected as the target gene because its partial sequence of cDNA was recently cloned from L. polyphemus brain in our laboratory (Cao et al., 1998). A 419-bp fragment of nonhomologous sequence derived from putative PKCepsilon and a 306-bp fragment from plasmid pUC 18 were generated for use as target and competitor in PCR MIMIC, respectively. 5. Within the genomic library DNA, a 0.8 value was obtained for the copy number of the putative PKCepsilon gene that was detected in 0.1 amol of one equivalent L. polyphemus genome in terms of the average recombinant molecular weight. In the genomic DNA, a single copy of putative PKCepsilon was found in 0.1 amol of one coverage for the L. polyphemus genome. Thus, it was implied that nearly 80% genetic resource was incorporated into the library. This percentage was termed the incorporation rate. 6. Based on these findings, we suggest that the incorporation rate is an essential factor for evaluating genomic libraries, particularly, when using partial digestion with restriction enzymes for library construction.
doi_str_mv 10.1023/A:1007027232412
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A lambda phage genomic DNA library for Limulus (L.) polyphemus brain was constructed using the AGEM-12 vector and the host strain KW251. 2. The primary library contained approximately 1.275 x 10(6) independent clones, increasing upon amplfication to 6.66 x 10(9) pfu/ml in a total volume of 58 ml. 3. A total of 28 clones was randomly chosen for a determination of the average size of inserts in the library. All clones contained inserts and the average size was 14.9 kb, ranging from 11.7 to 28.0 kb. The library provides a 10-fold equivalent of the L. polyphemus genome. 4. A new approach for evaluating a genomic DNA library was developed, in which competitive PCR MIMIC was employed to determine the target gene copy number in both constructed library and brain genomic DNA. The putative protein kinase C epsilon (PKCepsilon) was selected as the target gene because its partial sequence of cDNA was recently cloned from L. polyphemus brain in our laboratory (Cao et al., 1998). 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A lambda phage genomic DNA library for Limulus (L.) polyphemus brain was constructed using the AGEM-12 vector and the host strain KW251. 2. The primary library contained approximately 1.275 x 10(6) independent clones, increasing upon amplfication to 6.66 x 10(9) pfu/ml in a total volume of 58 ml. 3. A total of 28 clones was randomly chosen for a determination of the average size of inserts in the library. All clones contained inserts and the average size was 14.9 kb, ranging from 11.7 to 28.0 kb. The library provides a 10-fold equivalent of the L. polyphemus genome. 4. A new approach for evaluating a genomic DNA library was developed, in which competitive PCR MIMIC was employed to determine the target gene copy number in both constructed library and brain genomic DNA. The putative protein kinase C epsilon (PKCepsilon) was selected as the target gene because its partial sequence of cDNA was recently cloned from L. polyphemus brain in our laboratory (Cao et al., 1998). A 419-bp fragment of nonhomologous sequence derived from putative PKCepsilon and a 306-bp fragment from plasmid pUC 18 were generated for use as target and competitor in PCR MIMIC, respectively. 5. Within the genomic library DNA, a 0.8 value was obtained for the copy number of the putative PKCepsilon gene that was detected in 0.1 amol of one equivalent L. polyphemus genome in terms of the average recombinant molecular weight. In the genomic DNA, a single copy of putative PKCepsilon was found in 0.1 amol of one coverage for the L. polyphemus genome. Thus, it was implied that nearly 80% genetic resource was incorporated into the library. This percentage was termed the incorporation rate. 6. Based on these findings, we suggest that the incorporation rate is an essential factor for evaluating genomic libraries, particularly, when using partial digestion with restriction enzymes for library construction.</description><subject>Animals</subject><subject>Bacteriophage lambda - genetics</subject><subject>Brain Chemistry - genetics</subject><subject>DNA - analysis</subject><subject>DNA libraries</subject><subject>Genomic Library</subject><subject>Horseshoe Crabs - genetics</subject><subject>Horseshoe Crabs - metabolism</subject><subject>Lambda Phage</subject><subject>Limulus polyphemus</subject><subject>Polymerase Chain Reaction</subject><issn>0272-4340</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2000</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNqFkL1PwzAUxD2AaCnMbMgTW-A922lStqp8ShUgVMQY2c5zaxQ3IU4q8d-TCpiZ7oafTnfH2BnCJYKQV_NrBMhAZEIKheKAjfc-UVLBiB3H-AEAM4D0iI1wMCgyGLP31YZ4H4nXjts6NNT5zu-IvyxeefDBW97VnHa66nVHXPOlD33VR17pYErNm41eE1_Ttt6jN09zXnnT6vbrhB06XUU6_dUJe7u7XS0ekuXz_eNivkysyFWXmBxxBkoN1XLMyAqRpqI0udWSNOXT0gqHQisadlHqsDTO5s7oUpZ5ah3JCbv4yW3a-rOn2BXBR0tVpbdU97HIUExBIf4LYjYFKdN0AM9_wd4EKoum9WEYVPx9Jr8Bn7trVQ</recordid><startdate>20000801</startdate><enddate>20000801</enddate><creator>Wang, Y</creator><creator>Cao, Z</creator><creator>Reid, E A</creator><creator>Newkirk, R F</creator><creator>Ivy, M T</creator><creator>Townsel, J G</creator><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>7TK</scope><scope>7X8</scope></search><sort><creationdate>20000801</creationdate><title>The use of competitive PCR mimic to evaluate a Limulus lambda phage genomic DNA library</title><author>Wang, Y ; Cao, Z ; Reid, E A ; Newkirk, R F ; Ivy, M T ; Townsel, J G</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c284t-b8119044000817ec22552db8ca3eae86dc2f12a4e702e5f1dbfc8fbad3d85cfe3</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2000</creationdate><topic>Animals</topic><topic>Bacteriophage lambda - genetics</topic><topic>Brain Chemistry - genetics</topic><topic>DNA - analysis</topic><topic>DNA libraries</topic><topic>Genomic Library</topic><topic>Horseshoe Crabs - genetics</topic><topic>Horseshoe Crabs - metabolism</topic><topic>Lambda Phage</topic><topic>Limulus polyphemus</topic><topic>Polymerase Chain Reaction</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Wang, Y</creatorcontrib><creatorcontrib>Cao, Z</creatorcontrib><creatorcontrib>Reid, E A</creatorcontrib><creatorcontrib>Newkirk, R F</creatorcontrib><creatorcontrib>Ivy, M T</creatorcontrib><creatorcontrib>Townsel, J G</creatorcontrib><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>Neurosciences Abstracts</collection><collection>MEDLINE - Academic</collection><jtitle>Cellular and molecular neurobiology</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Wang, Y</au><au>Cao, Z</au><au>Reid, E A</au><au>Newkirk, R F</au><au>Ivy, M T</au><au>Townsel, J G</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>The use of competitive PCR mimic to evaluate a Limulus lambda phage genomic DNA library</atitle><jtitle>Cellular and molecular neurobiology</jtitle><addtitle>Cell Mol Neurobiol</addtitle><date>2000-08-01</date><risdate>2000</risdate><volume>20</volume><issue>4</issue><spage>509</spage><epage>520</epage><pages>509-520</pages><issn>0272-4340</issn><abstract>1. A lambda phage genomic DNA library for Limulus (L.) polyphemus brain was constructed using the AGEM-12 vector and the host strain KW251. 2. The primary library contained approximately 1.275 x 10(6) independent clones, increasing upon amplfication to 6.66 x 10(9) pfu/ml in a total volume of 58 ml. 3. A total of 28 clones was randomly chosen for a determination of the average size of inserts in the library. All clones contained inserts and the average size was 14.9 kb, ranging from 11.7 to 28.0 kb. The library provides a 10-fold equivalent of the L. polyphemus genome. 4. A new approach for evaluating a genomic DNA library was developed, in which competitive PCR MIMIC was employed to determine the target gene copy number in both constructed library and brain genomic DNA. The putative protein kinase C epsilon (PKCepsilon) was selected as the target gene because its partial sequence of cDNA was recently cloned from L. polyphemus brain in our laboratory (Cao et al., 1998). A 419-bp fragment of nonhomologous sequence derived from putative PKCepsilon and a 306-bp fragment from plasmid pUC 18 were generated for use as target and competitor in PCR MIMIC, respectively. 5. Within the genomic library DNA, a 0.8 value was obtained for the copy number of the putative PKCepsilon gene that was detected in 0.1 amol of one equivalent L. polyphemus genome in terms of the average recombinant molecular weight. In the genomic DNA, a single copy of putative PKCepsilon was found in 0.1 amol of one coverage for the L. polyphemus genome. Thus, it was implied that nearly 80% genetic resource was incorporated into the library. This percentage was termed the incorporation rate. 6. Based on these findings, we suggest that the incorporation rate is an essential factor for evaluating genomic libraries, particularly, when using partial digestion with restriction enzymes for library construction.</abstract><cop>Netherlands</cop><pmid>10901270</pmid><doi>10.1023/A:1007027232412</doi><tpages>12</tpages></addata></record>
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subjects Animals
Bacteriophage lambda - genetics
Brain Chemistry - genetics
DNA - analysis
DNA libraries
Genomic Library
Horseshoe Crabs - genetics
Horseshoe Crabs - metabolism
Lambda Phage
Limulus polyphemus
Polymerase Chain Reaction
title The use of competitive PCR mimic to evaluate a Limulus lambda phage genomic DNA library
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