Direct sequencing of bacterial artificial chromosomes (BACs) and prokaryotic genomes by biotin-capture PCR

被引：10

作者：

Sterky, F ^{[1
]}

Holmberg, A ^{[1
]}

Alexandersson, G ^{[1
]}

Lundeberg, J ^{[1
]}

Uhlén, M ^{[1
]}

机构：

[1] Royal Inst Technol, KTH, Dept Biochem & Biotechnol, S-10044 Stockholm, Sweden

来源：

JOURNAL OF BIOTECHNOLOGY | 1998年 / 60卷 / 1-2期

关键词：

genome sequencing; biotin capture; solid-phase technology; PCF;

D O I：

10.1016/S0168-1656(97)00196-X

中图分类号：

Q81 [生物工程学（生物技术）]; Q93 [微生物学];

学科分类号：

071005 ; 0836 ; 090102 ; 100705 ;

摘要：

Determination of unknown DNA sequences adjacent to known segments is an important task in genome-related research. We have applied the methodology of biotin-capture PCR for direct sequencing of bacterial artificial chromosomes (BACs) and bacterial genomes. The strategy involves extension of a biotinylated primer from a known locus into unknown regions of the template to yield single-stranded DNA, which is immobilised onto paramagnetic beads. An arbitrary primer initiates extension from the unknown region and back towards the known locus. The arbitrary primer contains a universal primer 'handle', which is utilised for subsequent amplification. The PCR products are then directly sequenced by solid-phase or cycle sequencing. The fact that BACs or bacterial chromosomes can be sequenced without prior purification or subcloning might be useful in numerous applications, such as gap-filling, sequencing of regulatory regions upstream known genes and determination of intron/exon-boundaries. (C) 1998 Published by Elsevier Science B.V. All rights reserved.

引用

页码：119 / 129

页数：11

共 28 条

[1] UNKNOWN SEQUENCE AMPLIFICATION - APPLICATION TO INVITRO GENOME WALKING IN CHLAMYDIA TRACHOMATIS L2 [J].

COPLEY, CG ;

BOOT, C ;

BUNDELL, K ;

MCPHEAT, WL .

BIO-TECHNOLOGY, 1991, 9 (01) :74-79

[2] SPLINKERETTES IMPROVED VECTORETTES FOR GREATER EFFICIENCY IN PCR WALKING [J].

DEVON, RS ;

PORTEOUS, DJ ;

BROOKES, AJ .

NUCLEIC ACIDS RESEARCH, 1995, 23 (09) :1644-1645

[3]

ESPELUND M, 1992, BIOTECHNIQUES, V13, P74

[4] CLONING OF THE SHARK PO PROMOTER USING A GENOMIC WALKING TECHNIQUE BASED ON THE POLYMERASE CHAIN-REACTION [J].

FORS, L ;

SAAVEDRA, RA ;

HOOD, L .

NUCLEIC ACIDS RESEARCH, 1990, 18 (09) :2793-2799

[5] RAPID PRODUCTION OF FULL-LENGTH CDNAS FROM RARE TRANSCRIPTS - AMPLIFICATION USING A SINGLE GENE-SPECIFIC OLIGONUCLEOTIDE PRIMER [J].

FROHMAN, MA ;

DUSH, MK ;

MARTIN, GR .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (23) :8998-9002

[6]

HOLMBERG A, 1994, AUTOMATED DNA SEQUEN, P139

[7]

HULTMAN T, 1991, BIOTECHNIQUES, V10, P84

[8] DIRECT SOLID-PHASE SEQUENCING OF GENOMIC AND PLASMID DNA USING MAGNETIC BEADS AS SOLID SUPPORT [J].

HULTMAN, T ;

STAHL, S ;

HORNES, E ;

UHLEN, M .

NUCLEIC ACIDS RESEARCH, 1989, 17 (13) :4937-4946

[9] SEQUENCE SPECIFIC GENERATION OF A DNA PANHANDLE PERMITS PCR AMPLIFICATION OF UNKNOWN FLANKING DNA [J].

JONES, DH ;

WINISTORFER, SC .

NUCLEIC ACIDS RESEARCH, 1992, 20 (03) :595-600

[10]

Lagerstrom M, 1991, PCR Methods Appl, V1, P111

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