Analysis of NotI linking clones isolated from human chromosome 3 specific libraries
We have partially sequenced more than 1000 NotI linking clones isolated from human chromosome 3-specific libraries. Of these clones, 152 were unique chromosome 3-specific clones. The clones were precisely mapped using a combination of fluorescence in situ hybridization (FISH) and hybridization to so...
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Published in | Gene Vol. 239; no. 2; pp. 259 - 271 |
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Main Authors | , , , , , , , , , , , , , , , , , , , , , , , |
Format | Journal Article |
Language | English |
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Netherlands
Elsevier B.V
01.11.1999
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Abstract | We have partially sequenced more than 1000
NotI linking clones isolated from human chromosome 3-specific libraries. Of these clones, 152 were unique chromosome 3-specific clones. The clones were precisely mapped using a combination of fluorescence in situ hybridization (FISH) and hybridization to somatic cell or radiation hybrids. Two- and three-color FISH was used to order the clones that mapped to the same chromosomal region, and in some cases, chromosome jumping was used to resolve ambiguous mapping. When this
NotI restriction map was compared with the yeast artificial chromosome (YAC) based chromosome 3 map, significant differences in several chromosome 3 regions were observed. A search of the EMBL nucleotide database with these sequences revealed homologies (90–100%) to more than 100 different genes or expressed sequence tags (ESTs). Many of these homologies were used to map new genes to chromosome 3. These results suggest that sequencing
NotI linking clones, and sequencing CpG islands in general, may complement the EST project and aid in the discovery of all human genes by sequencing random cDNAs. This method may also yield information that cannot be obtained by the EST project alone; namely, the identification of the 5′ ends of genes, including potential promoter/enhancer regions and other regulatory sequences |
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AbstractList | We have partially sequenced more than 1000 NotI linking clones isolated from human chromosome 3-specific libraries. Of these clones, 152 were unique chromosome 3-specific clones. The clones were precisely mapped using a combination of fluorescence in situ hybridization (FISH) and hybridization to somatic cell or radiation hybrids. Two- and three-color FISH was used to order the clones that mapped to the same chromosomal region, and in some cases, chromosome jumping was used to resolve ambiguous mapping. When this NotI restriction map was compared with the yeast artificial chromosome (YAC) based chromosome 3 map, significant differences in several chromosome 3 regions were observed. A search of the EMBL nucleotide database with these sequences revealed homologies (90-100%) to more than 100 different genes or expressed sequence tags (ESTs). Many of these homologies were used to map new genes to chromosome 3. These results suggest that sequencing NotI linking clones, and sequencing CpG islands in general, may complement the EST project and aid in the discovery of all human genes by sequencing random cDNAs. This method may also yield information that cannot be obtained by the EST project alone; namely, the identification of the 5' ends of genes, including potential promoter/enhancer regions and other regulatory sequences We have partially sequenced more than 1000 NotI linking clones isolated from human chromosome 3-specific libraries. Of these clones, 152 were unique chromosome 3-specific clones. The clones were precisely mapped using a combination of fluorescence in situ hybridization (FISH) and hybridization to somatic cell or radiation hybrids. Two- and three-color FISH was used to order the clones that mapped to the same chromosomal region, and in some cases, chromosome jumping was used to resolve ambiguous mapping. When this NotI restriction map was compared with the yeast artificial chromosome (YAC) based chromosome 3 map, significant differences in several chromosome 3 regions were observed. A search of the EMBL nucleotide database with these sequences revealed homologies (90–100%) to more than 100 different genes or expressed sequence tags (ESTs). Many of these homologies were used to map new genes to chromosome 3. These results suggest that sequencing NotI linking clones, and sequencing CpG islands in general, may complement the EST project and aid in the discovery of all human genes by sequencing random cDNAs. This method may also yield information that cannot be obtained by the EST project alone; namely, the identification of the 5′ ends of genes, including potential promoter/enhancer regions and other regulatory sequences |
Author | Muravenko, O.V Zakharyev, V.M Zabarovska, V.I Winberg, G Kisselev, L.L Li, J Klein, G Braga, E.A Kost-Alimova, M Sumegi, J Zelenin, A.V Lerman, M Zabarovsky, E.R Protopopov, A.I Vorobieva, N.V Domninsky, D.A Sheer, D Wahlestedt, C Kashuba, V.I Kiss, C Gizatullin, R.Z Fedorova, L Allikmets, R Grafodatsky, A |
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Keywords | RFLP, restriction fragment length polymorphism NotI map FISH, fluorescence in situ hybridization YAC, yeast artificial chromosome PFGE, pulsed field gel electrophoresis PCR, polymerase chain reaction Gene mapping Gene discovery EST, expressed sequence tag CpG islands |
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Snippet | We have partially sequenced more than 1000
NotI linking clones isolated from human chromosome 3-specific libraries. Of these clones, 152 were unique chromosome... We have partially sequenced more than 1000 NotI linking clones isolated from human chromosome 3-specific libraries. Of these clones, 152 were unique chromosome... |
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SubjectTerms | Animals Cell Line Chromosome Mapping Chromosomes, Human, Pair 3 - genetics CpG islands Databases, Factual Deoxyribonucleases, Type II Site-Specific - metabolism DNA - chemistry DNA - genetics DNA - metabolism Expressed Sequence Tags Gene discovery Gene Library Gene mapping Humans Hybrid Cells In Situ Hybridization, Fluorescence Medicin och hälsovetenskap Mice NotI map Sequence Alignment Sequence Analysis, DNA |
Title | Analysis of NotI linking clones isolated from human chromosome 3 specific libraries |
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