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本文引用的文献

1
Direct demonstration and quantification of long-range DNA looping by the lambda bacteriophage repressor.通过λ噬菌体阻遏物对远距离DNA环化进行直接演示和定量分析。
Nucleic Acids Res. 2009 May;37(9):2789-95. doi: 10.1093/nar/gkp134. Epub 2009 Mar 10.
2
Atomic force microscopy of the EcoKI Type I DNA restriction enzyme bound to DNA shows enzyme dimerization and DNA looping.与DNA结合的EcoKI I型DNA限制酶的原子力显微镜观察显示出酶二聚化和DNA环化。
Nucleic Acids Res. 2009 Apr;37(6):2053-63. doi: 10.1093/nar/gkp042. Epub 2009 Feb 17.
3
Switches in bacteriophage lambda development.噬菌体λ发育中的转换
Annu Rev Genet. 2005;39:409-29. doi: 10.1146/annurev.genet.39.073003.113656.
4
Determination of protein-DNA binding constants and specificities from statistical analyses of single molecules: MutS-DNA interactions.通过单分子统计分析确定蛋白质 - DNA 结合常数和特异性:MutS - DNA 相互作用
Nucleic Acids Res. 2005 Aug 1;33(13):4322-34. doi: 10.1093/nar/gki708. Print 2005.
5
Revisited gene regulation in bacteriophage lambda.噬菌体λ中基因调控的再探讨
Curr Opin Genet Dev. 2005 Apr;15(2):145-52. doi: 10.1016/j.gde.2005.02.001.
6
Design and validation of a tool for neurite tracing and analysis in fluorescence microscopy images.荧光显微镜图像中神经突追踪与分析工具的设计与验证
Cytometry A. 2004 Apr;58(2):167-76. doi: 10.1002/cyto.a.20022.
7
Cooperativity in long-range gene regulation by the lambda CI repressor.λ CI 阻遏蛋白在远距离基因调控中的协同作用。
Genes Dev. 2004 Feb 1;18(3):344-54. doi: 10.1101/gad.1167904.
8
Structure of a ternary transcription activation complex.三元转录激活复合物的结构
Mol Cell. 2004 Jan 16;13(1):45-53. doi: 10.1016/s1097-2765(03)00483-0.
9
Protein-protein and protein-DNA interactions of sigma70 region 4 involved in transcription activation by lambdacI.参与λcI转录激活的σ70区域4的蛋白质-蛋白质和蛋白质-DNA相互作用。
J Mol Biol. 2002 Nov 15;324(1):17-34. doi: 10.1016/s0022-2836(02)01043-4.
10
Octamerization of lambda CI repressor is needed for effective repression of P(RM) and efficient switching from lysogeny.λ CI 阻遏蛋白的八聚化对于有效抑制 P(RM) 和从溶原状态高效转换是必需的。
Genes Dev. 2001 Nov 15;15(22):3013-22. doi: 10.1101/gad.937301.

λ阻遏蛋白寡聚体固定DNA环的原子力显微镜研究

AFM studies of lambda repressor oligomers securing DNA loops.

作者信息

Wang Haowei, Finzi Laura, Lewis Dale E A, Dunlap David

机构信息

Department of Cell Biology, Emory University, Atlanta, GA 30322, USA.

出版信息

Curr Pharm Biotechnol. 2009 Aug;10(5):494-501. doi: 10.2174/138920109788922155.

DOI:10.2174/138920109788922155
PMID:19689317
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3641193/
Abstract

Large, cooperative assemblies of proteins that wrap and/or loop genomic DNA may "epigenetically" shift configurational equilibria that determine developmental pathways. Such is the case of the lambda bacteriophage which may exhibit virulent (lytic) or quiescent (lysogenic) growth. The lysogenic state of lambda prophages is maintained by the lambda repressor (CI), which binds to tripartite operator sites in each of the O(L) and O(R) control regions located about 2.3 kbp apart on the phage genome and represses lytic promoters. Dodd and collaborators have suggested that an initial loop formed by interaction between CI bound at O(R) and O(L) provides the proper scaffold for additional CI binding to attenuate the P(RM) promoter and avoid over production of CI. Recently, the looping equilibrium as a function of CI concentration was measured using tethered particle motion analysis, but the oligomerization of CI in looped states could not be determined. Scanning force microscopy has now been used to probe these details directly. An equilibrium distribution of looped and unlooped molecules confined to a plane was found to be commensurate to that for tethered molecules in solution, and the occupancies of specific operator sites for several looped and unlooped conformations were determined. Some loops appeared to be sealed by oligomers of 6-8, most by oligomers of 10-12, and a few by oligomers of 14-16.

摘要

包裹和/或环绕基因组DNA的大型蛋白质协作组装体可能会“表观遗传地”改变决定发育途径的构型平衡。λ噬菌体就是这样的例子,它可能表现出烈性(裂解性)或静止(溶原性)生长。λ原噬菌体的溶原状态由λ阻遏蛋白(CI)维持,CI与噬菌体基因组上相隔约2.3 kbp的O(L)和O(R)每个控制区域中的三方操纵位点结合,并抑制裂解启动子。多德及其合作者提出,由结合在O(R)和O(L)上的CI之间相互作用形成的初始环为额外的CI结合提供了合适的支架,以减弱P(RM)启动子的活性并避免CI的过量产生。最近,利用系留粒子运动分析测量了作为CI浓度函数的环化平衡,但无法确定环化状态下CI的寡聚化情况。现在已经使用扫描力显微镜直接探测这些细节。发现局限于平面的环化和未环化分子的平衡分布与溶液中系留分子的平衡分布相当,并确定了几种环化和未环化构象的特定操纵位点的占有率。一些环似乎由6 - 8聚体封闭,大多数由10 - 12聚体封闭,少数由14 - 16聚体封闭。