高效、新T-DNA侧翼序列分离技术--Actail-PCR 被引量：4

Actail-PCR—A New and Efficient Procedure for Isolation of Unknown Target Sequences Adjacent to T-DNA Border

下载PDF

导出

摘要【目的】建立一种有效分离T-DNA插入突变体侧翼基因组序列的方法。【方法】分离侧翼的目标基因组序列是利用T-DNA标签法研究植物功能基因组学的一个关键步骤,笔者发展稳定高效的Actail-PCR分离技术。该技术一侧引物来自于T-DNA载体,另一侧引物为一个复性控制引物。复性控制引物在3'端为一个14bp的随机简并引物,在5'端非目标尾部序列接上一个通用引物,中间由5个多聚脱氧次黄嘌呤核苷(poly(dI))连接。【结果】Actail-PCR技术将随机简并引物重新编辑成复性控制引物,在40℃的低严谨条件下,3'端的随机简并引物可以与T-DNA插入突变体的侧翼目标区段随机的结合,扩增得到目标片段,随后利用5'端的通用引物与T-DNA载体上的巢式引物依次组合,在65℃(10个循环后逐步降温至58℃)的高严谨条件下逐步扩增特异片段,同时抑制非特异性扩增,可以显著提高目标片段的扩增效率,减少假阳性。【结论】相对传统的TAIL-PCR,Actail-PCR技术可以更高效地分离T-DNA插入突变体的侧翼基因组序列。【Objective】 This study aimed at establishing a protocol to identify unknown target sequences adjacent to T-DNA borders. 【Method】 DNA tagging by T-DNA insertions has become an important approach for study of functional genomics in plants. To identify the genes tagged by T-DNA insertions, a novel and efficient procedure,named as annealing control thermal asymmetric interlaced PCR （Actail-PCR）, was developed to isolate genomic sequences flanking the insertion tags. In this procedure, four nested sequence-specific primers from T-DNA were utilized. The other side primer was a annealing control primer （ACP）, which comprises a tripartite structure with a polydeoxyinosine （poly （dI）） linker between the 3＇ end shorter arbitrary degenerated primer sequence （AD） and the 5＇ end nontarget universal sequence. 【Result】 Annealing control primers were designed for Actail-PCR instead of shorter arbitrary degenerated primers of TAIL-PCR. At 40℃ low stringency, PCR cycle was conducted to create one or more annealing sites for the AD primer along the target sequence like TAIL-PCR, and then, target products were preferentially amplified over 5＇ end nontarget universal primer and nested sequence-specific primers from T-DNA at 65℃ （after 10 cycles, annealing temperature droped to 58℃） high-stringency, so the efficiency and specificity of PCR amplification were greatly improved. 【Conclusion】 An novel procedure for isolation of unknown target sequences adjacent to T-DNA in the rice has been established. Actail-PCR is more efficient and useful for identification of the genes tagged by T-DNA insertions

作者杨立勇刘灶长周立国罗华程罗利军

机构地区上海市农业生物基因中心/作物遗传改良国家重点实验室种质资源分室(上海) 华中农业大学

出处《中国农业科学》 CAS CSCD 北大核心 2009年第4期1447-1451,共5页 Scientia Agricultura Sinica

基金上海市浦江人才计划(05PJ14085) 上海市重大基础研究计划(03DJ14015,05DJ14008) 农青科技2008(01)

关键词 T-DNA 侧翼序列 TAIL-PCR Actail-PCR T-DNA flank sequence TAIL-PCR Actail-PCR

分类号 Q78 [生物学—分子生物学]

引文网络
相关文献

参考文献13

1Jeon J S, Lee S, Lee S, Yang K, Choi J H, Cho Jung K H, Jo.n S H, Jeong D H, Lee J, Kim C, Jang S, Nam J, An K, Hart M J, Sung R, Choi H S, Yu J H, S Y, Cha S S, Kim S I, An G. T-DNA insertional mutagenesis for functional genomics in rice. Plant Journal, 2000, 22 561-570. 被引量：1
2Sessions A, Burke E, Presting G, Aux G, McElver J, Patton D, Dietrich B, Ho P, Bacwaden J, Ko C, Clarke J D, Cotton D, Bullis D, Snell J, Miguel T, Hutchison D, Kimmerly B, Mitzel T, Katagiri F, Glazebrook J, Law M, Goff S A. A high-throughput Arabidopsis reverse genetics system. Plant Cell, 2002, 14: 2985-2994. 被引量：1
3Liu Y G, Whittler R E Thermal asymmetric interlaced PCR: automatable amplification and sequencing of insert end fragments from PI and YAC clones for chromosome walking. Genome, 1995, 25: 674-681. 被引量：1
4Liu Y G, Mitsukawa N, Oosumi T, Whittier R F. Efficient isolation and mapping of Arabidopsis thaliana T-DNA insert junctions by thermal asymmetric interlaced PCR. Plant Journal, 1995, 8: 457-463. 被引量：1
5Liu Y G, Huang N. Efficient amplification of insert end sequences from bacterial artificial chromosome clones by thermal asymmetric interlaced PCR. Plant Molecular Biology Reporter, 1998, 16:175-181. 被引量：1
6Brownie J, Shawcross S, Theaker J, Whitcombe D, Ferrie R, Newton C, Little S. The elimination of primer-dimer accumulation in PCR. Nucleic Acids Research, 1997, 25: 3235-3241. 被引量：1
7Ailenberg M, Silverman M. specificity in carrying out incorporated primers (TULIPS) Controlled hot start and improved PCR utilizing touch-up and loop Biotechniques, 2000, 29:1018-1024. 被引量：1
8Hwang I T, Kim Y J, Kim S H, Kwak C I, Gu Y Y, Chun J Y. Annealing control primer system for improving specificity of PCR amplification. Biotechniques, 2003, 35(6): 1180-1184. 被引量：1
9Kim Y J, Kwak C I, Gu Y Y, Hwang I T, Chun J Y. Annealing control primer system for identification of differentially expressed genes on agarose gels. Biotechniques, 2004, 36(3): 424-430. 被引量：1
10Martin F H, Caslro M M, Aboulela F, Tinoeo I. Base pairing involving deoxyinosine: implication for probe design. Nucleic Acids Research, 1985, 13: 8927-8938. 被引量：1

二级参考文献94

1Antal Z.,Rascle C.,Fevre M.,and Bruel C.,2004,Single oligonucleotide nested PCR:a rapid method for the isolation of genes and their flanking regions from expressed sequence tags,Curr.Genet.,46:240-246 被引量：1
2Balzergue S.,Dubreucq B.,Chauvin S.,Le-Clainche I.,Le Boulaire F.,de Rose R.,Samson1 F.,Biaudet V.,Lechamy A.,Cruaud C.,Weissenbach J.,Caboche M.,and Lepiniec L.,2001,Improved PCR-Walking for large-scale isolation of plant T-DNA borders,Biotechniques,30:496-504 被引量：1
3Carmody M.W.,Jones M.,Tarraza H.,and Vary C.P.,1996,Use of the polymerase chain reaction to specifically amplify integrated HPV-16 DNA by virtue of its linkage to interspersed repetitive DNA,Mol.Cell Probes,10:107-116 被引量：1
4Cottage A.,Yang A.P.,Maunders H.,de Lacy R.C.,and Ramsay N.A.,2001,Identification of DNA sequences flanking T-DNA insertions by PCR-Walking,Plant Mol.Biol.Rep.,19:321-327 被引量：1
5Courcoul M.,Patience C.,Rey F.,Blanc D.,Harmache A.,and Sire J.,1995,Peripheral blood mononuclear cells produce normal amounts of defective Vif-human immunodeficiency virus type 1 particles which are restricted for the preretrotranscription steps,J.Virol.,69:2068-2074 被引量：1
6Devic M.,Albert S.,Delseny M.,and Roscoe T.J.,1997,Efficient PCR walking on plant genomic DNA,Plant Physiol.Biochem.,35:331-339 被引量：1
7Devon R.S.,Porteous D.J.,and Brookes A.J.,1995,Spilinkerettes improved vectorettes for greater efficiency in PCR walking,Nucl.Acid.Res.,23:1644-1645 被引量：1
8Don R.H.,Cox P.T.,Wainwright B.J.,Baker K.,and Mattick J.S.,1991,Touchdown PCR to circumvent spurious priming during gene amplification,Nucl.Acid.Res.,19:4008 被引量：1
9Hecker K.H.,and Roux K.H.,1996,High and low annealing temperatures increase both specificity and yield in touchdown and stepdown PCR,Biotechniques,20:478-485 被引量：1
10Huang G.,Zhang L.,and Birch R.G.,2000,Rapid amplifcation and cloning of Tn5 flanking fragments by inverse PCR,Lett.Appl.Microbiol.,31:149-153 被引量：1

共引文献46

1杨坤,吴学龙,朗春秀,陈锦清.Isolation of the Flanking Sequences Adjacent to Transgenic T-DNA in Brassica napus Genome by an Improved Inverse PCR Method[J].Agricultural Science & Technology,2010,11(2):65-68. 被引量：2
2巢伟,刘永杰,陆承平.基因组步移技术扩增嗜水气单胞菌J-1株脂酶基因全长及原核表达[J].动物医学进展,2010,31(9):1-6. 被引量：1
3仇有文,高学军,张明辉,敖金霞,袁肖寒,刘营.抗除草剂转基因大豆插入拷贝数及其旁侧序列分析[J].生物技术,2011,21(6):31-35. 被引量：7
4唐存多,赵顺阁,邬敏辰,史红玲.宇佐美曲霉中β-甘露聚糖酶基因调控序列的克隆[J].食品与生物技术学报,2012,31(2):152-158.
5王葵娣,郑服丛.一种快速·有效分离T-DNA插入位点的侧翼序列的方法——DW-ACP-PCR技术[J].安徽农业科学,2007,35(28):8817-8818.
6王葵娣,林春花,郑服丛.稻瘟病菌突变体Y34-0453的表型分析和T-DNA插入位点的定位[J].热带作物学报,2008,29(1):58-63.
7龙海涛,李洪清,李玲.蓝猪耳启动子捕获系统的建立[J].北方园艺,2008(5):181-184. 被引量：2
8段继强,杜光辉,李建永,梁雪妮,刘飞虎.苎麻atp6和atp9基因的克隆表达及与细胞质雄性不育的相关性[J].遗传,2008,30(11):1487-1498. 被引量：12
9江贤章,陈金卿,田宝玉,高媛媛,舒正玉,李欣,蓝灿华,黄建忠.破囊壶菌Δ~4-脂肪酸脱饱和酶基因5'端侧翼区域的克隆与鉴定[J].福建师范大学学报（自然科学版）,2008,24(6):89-94. 被引量：4
10段继强,李建永,杜光辉,梁雪妮,刘飞虎.苎麻线粒体基因CoxⅡ和atpA与细胞质雄性不育相关性分析[J].中国农业科学,2009,42(2):434-445. 被引量：13

同被引文献64

1郑宗明,顾晓波,俞海青,梁凤来,刘如林.非核糖体肽合成酶主要结构域的研究进展[J].中国抗生素杂志,2005,30(2):120-124. 被引量：19
2李树林,周志疆,周熙荣.油菜显性核不育三系法制种[J].上海农业学报,1995,11(1):21-26. 被引量：29
3王汉中.中国油料产业发展的现状、问题与对策[J].中国油料作物学报,2005,27(4):100-105. 被引量：146
4李树林.甘蓝型油菜细胞核雄性不育性的遗传规律探讨及其应用[J].上海农业学报,1985,1(2):1-12. 被引量：13
5Lu G Y, Yang G S, Fu T D. Molecular mapping of a dominant genic male sterility gene ( Ms ) in rapeseed (Brasslca napus) [J]. Plant breeding, 2004,123 (3): 262 - 265. 被引量：1
6Huang Z, Chen Y, Yi B, et al. Fine mapping of the reces- sive genic male sterility gene (Brans3) in Brassica napus L. [ J]. Theor Appl Genet,2007,115 ( 1 ) : 113 - 118. 被引量：1
7Xiao L, Yi B, Chen Y, et al. Molecular markers linked to Bn;rf: a recessive epistatic inhibitor gene of recessive genic male sterility in Brassica napus L. [ J]. Euphytica, 2008,164(2) :377 -384. 被引量：1
8Paran I, Michelmore R W. Development of reliable PCR - based markers linked to downy mildew resistance genes in lettuce [ J ]. Theor Appl Genet, 1993,85 : 985 - 993. 被引量：1
9李春艳,张幸果,王同华,李媛媛,陈庆芳,傅廷栋,沈金雄,马朝芝.甘蓝型油菜自交不亲和临保性及其连锁AFLP标记[J].作物学报,2007,33(9):1452-1457. 被引量：3
10Leoni C, Volpicella M, DeLeo F, et al.. Genome walking in eukaryotes [J]. FEBS J., 2011, 278 (21) : 3953 -3977. 被引量：1

引证文献4

1杨立勇,刘灶长,周熙荣,王伟荣,李延莉,蒋美艳,孙超才.与甘蓝型油菜隐性核不育rf基因连锁标记的开发[J].中国油料作物学报,2011,33(3):216-220. 被引量：2
2李旭娟,陈杨玲,王海波,龚明,邹竹荣.基于PCR的非酶连型基因组步移技术研究进展[J].中国农业科技导报,2013,15(2):193-199. 被引量：1
3刘洋,柯晓静,于宏伟,郭润芳.一种新型抗菌肽基因决定簇的克隆与序列结构特征[J].河北农业大学学报,2019,42(1):65-70. 被引量：1
4马雪萌,余成敏,赛小玲,刘贞,桑海洋,崔百明.PSORA:一种基于高通量测序的T-DNA插入位点分析方法[J].中国农业科学,2022,55(15):2875-2882. 被引量：1

二级引证文献5

1黄团,黄先群,侯国佐,侯燕,李丽.油菜核不育系827AB育性基因的SRAP标记[J].贵州农业科学,2011,39(12):9-11. 被引量：1
2李延莉,杨立勇,王伟荣,蒋美艳,周熙荣,孙超才.高含油量隐性核不育杂交油菜新品种‘沪油杂6号'的选育[J].上海农业学报,2013,29(5):109-111. 被引量：1
3刘欣,魏小雅,于宏伟,郭润芳.非核糖体肽合成酶腺苷化结构域在E.coli中的表达及底物特异性分析[J].河北农业大学学报,2020,43(1):110-115.
4郝振凯,汤新明,张媛媛,谢福杰,陈君敏,索静霞,索勋,刘贤勇.利用二代测序技术对柔嫩艾美耳球虫T-DNA整合位点的分析及鉴定[J].中国农业大学学报,2023,28(8):183-190.
5高俊平.基因组步移技术概述[J].生物学教学,2019,44(3):77-79. 被引量：2

1天气多变化您会担心吗?——麦极除草稳定高效[J].湖北植保,2010(5):48-48.
2李小萍,汪敏,赵杨,丁胜利,李洪连,马宗斌.棉花黄萎病菌致病相关基因的分离及敲除载体的构建[J].河南农业大学学报,2015,49(6):787-793.
3扬州大学成功培育转基因糯稻新品种[J].种业导刊,2009(9):44-44.
4转基因糯稻新品种培育成功[J].农家致富,2009(18):19-19.
5方进,翟文学,王文明,李素文,朱立煌.转基因水稻T-DNA侧翼序列的扩增与分析[J].Acta Genetica Sinica,2001,28(4):345-351. 被引量：20
6JamesD.Metzger,Z.L.Zheng,李兴军,李三玉.植物功能基因组学[J].农业科技译丛（杭州）,2000(2):24-28.
7唐忠海,覃静萍,储成才,彭国平,饶力群.T-DNA标签法在水稻功能基因组研究中的应用[J].杂交水稻,2005,20(6):1-3.
8简讯[J].扬州大学学报（农业与生命科学版）,2007,28(2).
9扬大成功培育转基因糯稻新品种[J].北京农业（中旬刊）,2009,0(9):13-13.
10王翾宇.电石炉翻电石的原因及处理[J].化工管理,2014(12):42-42. 被引量：1

中国农业科学

2009年第4期

浏览历史

内容加载中请稍等...