美洲黑杨PdZFR基因的克隆和分析

Cloning and Analyzing of Gene PdZFR from Populus deltoides

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摘要根据美洲黑杨PdZFR部分cDNA序列,采用拟基因组文库步行法和RACE克隆了该基因全长cDNA及基因组DNA,并对该基因的启动子、转录起始位点、内含子分布、剪切方式、编码的氨基酸序列和该基因在染色体上的分布位置进行了分析。组织或器官特异表达分析表明:该基因与植物发育相关。 The full length cDNA and genomic DNA of PdZFR were cloned from Populus deltoides by RACE and Visual Genome Library Walking methods respectively,according to its partial cDNA sequence.Meanwhile,the gene promoter,transcription initiation,intron and exon distribution,spice pattern,the amino acid sequence encoded and the location of this gene on chromosome were analyzed.The tissue or organ-specific expression analysis showed that this gene was related to plant development.

作者王大海苏晓华张冰玉黄秦军张香华

机构地区中国林业科学研究院林业研究所

出处《林业科学研究》 CSCD 北大核心 2010年第5期637-643,共7页 Forest Research

基金引进国际先进林业科学技术”948”创新重大项目“杨树RNAi载体构建、材性相关基因克隆及功能研究”(2006-4-C01) 国家973项目“速生优质杨树的聚合育种与分子改良”(No.2009CB119107)

关键词 PdZFR 美洲黑杨 RACE VGL-Walking TATABox CAATBox PdZFR Populus deltoides RACE VGL-Walking TATA Box CAAT Box

分类号 S792.11 [农业科学—林木遗传育种]

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参考文献17

1Peter K,Klaus F X M,Christian S H.Evaluation and classification of RING-finger domains encoded by the Arabidopsis genome[J].Genome Biology,2002,3(4):12-21.
2Freemont P S.The RING fi nger:a novel protein sequencemotif related to the zinc finger[J].Ann N Y Acad Sci,1993,68:4174–4192.
3Jackson P K,Eldridge A G,Freed E,et al.The lore of the RINGs:substrate recognitionand catalysis by ubiquitin ligases[J].Trends Cell Biol,2000,10:429-439.
4Freemont P S.Ubiquitination:RING for destruction[J].Curr Biol,2000,10:R84-R87.
5Lorick K L,Jensen J P,Fang S.RING fingers mediate ubiquitin-conjugating enzyme (E2)-dependent ubiquitination[J].Proc Natl Acad Sci USA,1999,96:11364-11369.
6Dong C H,Agarwal M,Zhang Y Y,et al.The negative regulator of plant cold responses,HOS1,is a RING E3 ligase that mediates the ubiquitinationand degradation of ICE1[J].Pans,2006,103(21):8281-8286.
7Yang X,Sun C,Hu Y,et al.Molecular cloning and characterization of a gene encoding RING zinc finger ankyrin protein from drought-tolerant Artemisia desertorum[J] J Biosci,2008,33:103–112.
8Schramm G,Bruchhaus I,Roeder T.A simple and reliable 5'-RACE approach[J].Nucleic Acids Res,2000,28:e96.
9Carl W D,Gabriela S.Dveksler PCR Primer:A Laboratory Mannual[M].New york:Cold Spring Harbor Laboratory Press,2003,359-389.
10Bertling W M,Beier F,Reichenberger E.Determination of 5' ends of specific mRNAs by DNA ligase-dependent amplification[J].PCR Methods Appl,1993,3:95-99.

二级参考文献41

1Terauchi R, Kahl G. Rapid isolation of promoter sequences by TAIL-PCR, the 5-flanking regions of Pal and Pgi genes from yams (Dioscorea). Mol Gen Genet, 2000, 263(3):554-560.
2Hwang 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.
3Kim 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.
4Triglia T, Peterson M G, Kemp D J. A procedure for in vitro amplification of DNA segments that lie outside the boundaries of known sequences. Nucleic Acids Res, 1998,16 (16): 8186.
5Rosenthal A, Winistorfer S C. PCR amplification techniques for chromosome walking. Trends Biotechnol, 1992, 10(1):44-48.
6Tsuei D J, Chen P J, Lai M Y, Chan D S, Yang C S, Chan J Y,Hsu T Y. Inverse polymerase chain reaction for cloning cellular sequences adjacent to integrated hepatitis B virus DNA in hapa-tocellular carcinomas. J Virol Methods, 1994, 49 (3):269-284.
7Takemoto S, Matsuoka M, Yamaguchi K, Takatsuki K. A novel diagnostic method of adult T-cell leukemia: monoclonal integration of human T-cell lymphotropic virus type I provirus DNA detected by inverse polymerase chain reaction. Blood, 1994, 84(9):3080 - 3085.
8Cavrois M, Wain-Hobson S, Wattel E. Stochastic events in the amplification of HTLV-I integration sites by linker-mediated PCR.Res Virol, 1995, 146(3):179-184.
9Ohshima K, Suzumiya J, Kato A, Tashiro K, Kikuchi M. ClonalHTLV-I-infected CD4+ T-lymphocytes and non-clonal non-HTLV-I-infected giant cells in incipient ATLL with Hodgkin-like histologic features. Intl J Concer, 1997, 72(4):592-598.
10Ohshlma K, Mukai Y, Shiraki H, Suzumiya J, Tashiro K, Kikuchi M. Clonal integration and expression of human T-celt lymphotropic virus type I in carriers detected by polymerase chain reaction and inverse PCR. Am J Hematol, 1997, 54(4):306-312.

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1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
2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
3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.
4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.
5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
6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
7杨立勇,刘灶长,周立国,罗华程,罗利军.高效、新T-DNA侧翼序列分离技术--Actail-PCR[J].中国农业科学,2009,42(4):1447-1451. 被引量：4
8刘春香.基于随机引物的PCR-Walking技术[J].安徽农业科学,2010,38(6):2833-2835. 被引量：3
9王晓波,蒋凌雪,魏利,刘林,陆伟,李文欣,王俊,陶波,常汝镇,邱丽娟.外源抗草甘膦EPSPs基因在大豆基因组中的整合与定位[J].作物学报,2010,36(3):365-375. 被引量：13
10刘春香,张卫华,孙小镭.基于PCR的染色体步移中单引物扩增的克服与非特异引物的利用[J].中国生物化学与分子生物学报,2010,26(4):380-385. 被引量：1

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2刘凯,杨世湖,陈苗苗,李江涛,万建民.pib基因启动子3'端缺失体的暗诱导特性分析[J].农业生物技术学报,2010,18(4):630-637. 被引量：2
3张霞,宋瑞清,邓勋.黑木耳YBS-3菌株ras启动子的克隆与分析[J].安徽农业科学,2011,39(17):10130-10132. 被引量：1
4乌云塔娜,王淋,叶生晶.杜仲EuACOTS基因家族的鉴定及生物信息学分析[J].经济林研究,2013,31(4):1-8. 被引量：4
5高水平,范丙友,史国安,贾小平,孔祥生.矮牵牛CHS基因启动子克隆、序列分析及植物表达载体构建[J].北方园艺,2010(17):155-158. 被引量：4
6田奇琳,林玉玲,赖钟雄,王天池.龙眼胚性愈伤组织DlRan3A和DlRan3B基因启动子的克隆及其生物信息学分析[J].热带作物学报,2014,35(1):82-89. 被引量：7
7邓勋,宋小双,宋瑞清.姬松茸(Agaricus blazei Murrill.) gpd启动子的克隆及其序列分析[J].安徽农业科学,2009,37(3):993-995. 被引量：3
8张梅春,蔡萍,金刚.紫杉嫩枝扦插插穗处理的研究[J].辽宁林业科技,2006(5):29-30. 被引量：1
9耿立英,张传生,杜立新,陈红菊,沈萍,付志新.鸡cvh启动子调控的绿色荧光蛋白报告载体的构建及鉴定[J].中国农学通报,2009,25(3):13-17.
10张克,顾启光,曲宏成,刘力波,刘胜利,付春亮,耿炳伟.紫杉扦插繁育技术[J].辽宁林业科技,2001(6):44-45. 被引量：1

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美洲黑杨PdZFR基因的克隆和分析

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