A bacterial artificial chromosome transgenic mouse model for visualization of neurite growth 被引量：1

A bacterial artificial chromosome transgenic mouse model for visualization of neurite growth

导出

摘要 Class Ⅲ β-tubulin （Tubb3） is a component of the microtubules in neurons and contributes to microtubule dynamics that are required for axon outgrowth and guidance during neuronal development. We here report a novel bacterial artificial chromosome （BAC） transgenic mouse line that expresses Class Ⅲ β-tubulin fused to mCherry, an improved monomeric red fluorescent protein, for the visualization of microtubules during neuronal development. A BAC containing Tubb3 gene was modified by insertion of mCherry complementary DNA downstream of Tubb3 coding sequence via homologous recombination, mCherry fusion protein was expressed in the nervous system and testis of the transgenic animal, and the fluorescent signal was observed in the neurons that located in the olfactory bulb, cerebral cortex, hippocampal formation, cerebellum, as well as the retina. Besides, Tubb3-mCherry fusion protein mainly distributed in neurites and colocalized with endogenous Class Ⅲ β-tubulin The fusion protein labels Purkinje cell dendrites during cerebellar circuit formation. Therefore, this transgenic line might be a novel tool for scientific community to study neuronal development both in vitro and in vivo. Class III β-tubulin(Tubb3) is a component of the microtubules in neurons and contributes to microtubule dynamics that are required for axon outgrowth and guidance during neuronal development. We here report a novel bacterial artificial chromosome(BAC) transgenic mouse line that expresses Class III β-tubulin fused to m Cherry, an improved monomeric red fluorescent protein, for the visualization of microtubules during neuronal development. A BAC containing Tubb3 gene was modified by insertion of m Cherry complementary DNA downstream of Tubb3 coding sequence via homologous recombination. m Cherry fusion protein was expressed in the nervous system and testis of the transgenic animal, and the fluorescent signal was observed in the neurons that located in the olfactory bulb, cerebral cortex, hippocampal formation, cerebellum, as well as the retina. Besides, Tubb3-m Cherry fusion protein mainly distributed in neurites and colocalized with endogenous Class III β-tubulin. The fusion protein labels Purkinje cell dendrites during cerebellar circuit formation. Therefore, this transgenic line might be a novel tool for scientific community to study neuronal development both in vitro and in vivo.

作者 TAO Tao CHEN Chen SUN Jie PENG YaJing ZHU MinSheng

机构地区 Model Animal Research Center and MOE Key Laboratory of Model Animal for Disease Study

出处《Science China(Life Sciences)》 SCIE CAS CSCD 2015年第4期373-378,共6页 中国科学（生命科学英文版）

关键词 Tubb3 MCHERRY BAC transgenic mouse neuronal development Purkinje cells 转基因小鼠模型细菌人工染色体神经元发育轴突生长可视化微管蛋白红色荧光蛋白融合蛋白

分类号 Q42 [生物学—神经生物学]

引文网络
相关文献

参考文献18

1Dent EW, Gupton SL, Gertler FB. The growth cone cytoskeleton in axon outgrowth and guidance. Cold Spring Harb Perspect Biol, 2011, 3: pii: a001800.
2Ludin B, Matus A. GFP illuminates the cytoskeleton. Trends Cell Biol, 1998, 8: 72-77.
3Stepanova T, Slemmer J, Hoogenraad CC, Lansbergen G, Dortland B, De Zeeuw CI, Grosveld F, van Cappellen G, Akhmanova A, Galjart N. Visualization of microtubule growth in cultured neurons via the use of EB3-GFP (end-binding protein 3-green fluorescent protein). J Neurosci, 2003, 23: 2655-2664.
4Deinhardt K, Kim T, Spellman DS, Mains RE, Eipper BA, Neubert TA, Chao MV, Hempstead BL. Neuronal growth cone retraction relies on proneurotrophin receptor signaling through Rac. Sci Signal, 2011, 4: ra82.
5Riedl J, Flynn KC, Raducanu A, Gartner F, Beck G, Bosl M, Bradke F, Massberg S, Aszodi A, Sixt M, Wedlich-Soldner R. Lifeact mice for studying F-actin dynamics. Nat Meth, 2010, 7: 168-169.
6Sullivan KF. Structure and utilization of tubulin isotypes. Ann Rev Cell Biol, 1988, 4: 687-716.
7Lee MK, Rebhun LI, Frankfurter A. Posttranslational modification of class III beta-tubulin. Proc Natl Acad Sci USA, 1990, 87: 7195-7199.
8Tischfield MA, Baris HN, Wu C, Rudolph G, Van Maldergem L, He W, Chan WM, Andrews C, Demer JL, Robertson RL, Mackey DA, Ruddle JB, Bird TD, Gottlob I, Pieh C, Traboulsi EI, Pomeroy SL, Hunter DG, Soul JS, Newlin A, Sabol LJ, Doherty EJ, de Uzcátegui CE, de Uzcátegui N, Collins MLZ, Sener EC, Wabbels B, Hellebrand H, Meitinger T, de Berardinis T, Magli A, Schiavi C, Pastore-Trossello M, Koc F, Wong AM, Levin AV, Geraghty MT, Descartes M, Flaherty M, Jamieson RV, M?ller HU, Meuthen I, Callen DF, Kerwin J, Lindsay S, Meindl A, Gupta Jr ML, Pellman D, Engle EC. Human tubb3 mutations perturb microtubule dynamics, kinesin interactions, and axon guidance. Cell, 2010, 140: 74-87.
9Peng YJ, He WQ, Tang J, Tao T, Chen C, Gao YQ, Zhang WC, He XY, Dai YY, Zhu NC, Lv N, Zhang CH, Qiao YN, Zhao LP, Gao X, Zhu MS. Trio is a key guanine nucleotide exchange factor coordinating regulation of the migration and morphogenesis of granule cells in the developing cerebellum. J Biol Chem, 2010, 285: 24834-24844.
10Nogales E, Wolf SG, Downing KH. Structure of the αβ tubulin dimer by electron crystallography. Nature, 1998, 391: 199-203.

同被引文献11

1LIU Jing,LIANG XiJun,GAN ZhenJi.Transcriptional regulatory circuits controlling muscle fiber type switching[J].Science China(Life Sciences),2015,58(4):321-327. 被引量：3
2XU Na,SHEN Ning,WANG XiuXing,JIANG Shan,XUE Bin,LI ChaoJun.Protein prenylation and human diseases: a balance of protein farnesylation and geranylgeranylation[J].Science China(Life Sciences),2015,58(4):328-335. 被引量：4
3CAO Ying.Germ layer formation during Xenopus embryogenesis: the balance between pluripotency and differentiation[J].Science China(Life Sciences),2015,58(4):336-342. 被引量：2
4SHI WenChao,FANG ZhiBing,LI Li,LUO LingFei.Using zebrafish as the model organism to understand organ regeneration[J].Science China(Life Sciences),2015,58(4):343-351. 被引量：6
5LAN JianFeng,ZHANG Xuan,CHEN Di.Molecular mechanisms of dietary restriction in aging—insights from Caenorhabditis elegans research[J].Science China(Life Sciences),2015,58(4):352-358. 被引量：6
6ZOU JiangHuan,XIONG XiWen,LAI BeiBei,SUN Min,TU Xin,GAO Xiang.Glucose metabolic abnormality is associated with defective mineral homeostasis in skeletal disorder mouse model[J].Science China(Life Sciences),2015,58(4):359-367. 被引量：1
7QU ZhiPeng,WANG XiaoHan,LIU DongChuan,GAO Xiang,XU Ying.Inactivation of Cipc alters the expression of Per1 but not circadian rhythms in mice[J].Science China(Life Sciences),2015,58(4):368-372. 被引量：2
8LUO Jun,ZUO JunTao,WU Jing,WAN Ping,KANG Di,XIANG Cong,ZHU Hong,CHEN Jiong.In vivo RNAi screen identifies candidate signaling genes required for collective cell migration in Drosophila ovary[J].Science China(Life Sciences),2015,58(4):379-389. 被引量：1
9SUN Ye,MAO Ping,LU JingWei,DAI Jin,TENG HuaJian,JIANG Qing.ABO blood type and ABO gene with susceptibility to deep vein thrombosis following orthopedic surgery: a casecontrol study in Chinese Han population[J].Science China(Life Sciences),2015,58(4):390-391. 被引量：2
10QI Xin,GAO Xiang.Towards a better understanding of mouse and human diseases—International Mouse Phenotyping Consortium[J].Science China(Life Sciences),2015,58(4):392-395. 被引量：1

引证文献1

1GAO Xiang.Model animals and their applications[J].Science China(Life Sciences),2015,58(4):319-320. 被引量：7

二级引证文献7

1Ying Li,Gang Liu,Xin Lou,Zhiye Chen,Lin Ma.Intra-individual comparison of different gadolinium-based contrast agents in the quantitative evaluation of C6 glioma with dynamic contrast-enhanced magnetic resonance imaging[J].Science China(Life Sciences),2017,60(1):11-15. 被引量：4
2门可,段醒妹,杨阳,魏于全.基于CRISPR/Cas9基因编辑技术的人类遗传疾病基因治疗相关研究进展[J].中国科学：生命科学,2017,47(11):1130-1140. 被引量：3
3马宁,李正花,史季,乔瑜,王大勇,高旭.中国遗传改变小鼠研发与市场在近20年的发展与变化[J].科技导报,2019,37(14):51-58.
4Delia Gaskell,Mosleh Abualhaj.Advances in Gene Therapy for Human Genetic Diseases Based on Crispr/Cas9 Gene Editing Technology[J].Genetic Disease Study,2018,2(1):1-10.
5范小倩,韩雅洁,巩彩霞,赵子龙,乔成栋.CRISPR/Cas9基因编辑技术在阿尔茨海默病治疗中的研究现状[J].中国临床药理学杂志,2021,37(13):1749-1751.
6洪胜辉,卫振,刘平,许潇洒,倪利锋,王芊芊,丁潇,汪洌.高校外来基因工程小鼠质量控制技术分析与探讨[J].实验技术与管理,2022,39(7):224-227. 被引量：4
7汪斌,王倩.利用实验室病原微生物抽检控制实验动物质量[J].中南农业科技,2023,44(9):113-115. 被引量：1

1巩学千,陈受宜,龚继明,刘峰.Isolation and mapping of bacterial artificial chromosome (BAC) clone containing telomere-associated sequence[J].Science China(Life Sciences),1998,41(6):617-622.
2张忠诚.动物乳腺生物反应器的原理及研究进展[J].中国奶牛,2006(4):27-30. 被引量：7
3Fredrick J.Seil.Circuit reorganization in cerebellar cultures after injury[J].Neural Regeneration Research,2015,10(7):1045-1046.
4王起明,孙烨超,厉申捷,叶建平.白眉长臂猿基因组BAC文库的构建[J].绍兴文理学院学报,2015,35(10):13-15. 被引量：2
5Qiannan Wang,Shanjin Huang.Visualization of MicrotubuleOrganization and Dynamics in Living Arabidopsis Embryonic Cells[J].Molecular Plant,2014,7(8):1397-1401. 被引量：3
6Xuebiao Yao,Guowei Fang.Visualization and orchestration of the dynamic molecular society in cells[J].Cell Research,2009,19(2):152-155. 被引量：3
7MitsuhiroKawata.Nuclear receptor dynamics and GFP transgenic mouse[J].中国组织化学与细胞化学杂志,2004,13(3):333-334.
8Jing Wang,Honglin Xu,Yuqiang Jiang,Mikiko Takahashi,Masatoshi Takeichi,Wenxiang Meng.CAMSAP3-dependent microtubule dynamics regulates Golgi assembly in epithelial cells[J].Journal of Genetics and Genomics,2017,44(1):39-49.
9陈献伟,王会,关伟军,高剑峰.细菌人工染色体文库基因组DNA制备技术[J].中国畜牧兽医,2010,37(5):79-82. 被引量：1
10Huijun Xue Xin Xu Yu V. Fu.New insights in pre-replication complex formation with single-molecule visualization[J].Science Bulletin,2015,60(12):1133-1135. 被引量：2

Science China(Life Sciences)

2015年第4期

浏览历史

内容加载中请稍等...

A bacterial artificial chromosome transgenic mouse model for visualization of neurite growth 被引量：1

参考文献18

同被引文献11

引证文献1

二级引证文献7

相关作者

相关机构

相关主题

浏览历史