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本文引用的文献

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Molecular genetic truncation analysis of filament assembly and phosphorylation domains of Dictyostelium myosin heavy chain.盘基网柄菌肌球蛋白重链丝状体组装和磷酸化结构域的分子遗传截短分析
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2
The proteolytic substructure of light meromyosin. Localization of a region responsible for the low ionic strength insolubility of myosin.轻酶解肌球蛋白的蛋白水解亚结构。肌球蛋白低离子强度不溶性相关区域的定位。
J Biol Chem. 1983 Nov 10;258(21):13213-20.
3
Rigor crossbridge structure in tilted single filament layers and flared-X formations from insect flight muscle.来自昆虫飞行肌肉的倾斜单丝层和喇叭形-X 结构中的强直横桥结构。
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4
Disruption of the Dictyostelium myosin heavy chain gene by homologous recombination.通过同源重组破坏盘基网柄菌肌球蛋白重链基因。
Science. 1987 May 29;236(4805):1086-91. doi: 10.1126/science.3576222.
5
Invertebrate myosin filament: subfilament arrangement in the wall of tubular filaments of insect flight muscles.无脊椎动物肌球蛋白丝:昆虫飞行肌管状丝壁中的亚丝排列
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Expression in Escherichia coli of a functional Dictyostelium myosin tail fragment.功能性盘基网柄菌肌球蛋白尾部片段在大肠杆菌中的表达。
J Cell Biol. 1987 Dec;105(6 Pt 2):2999-3005. doi: 10.1083/jcb.105.6.2999.
7
Chemoattractant-elicited increases in Dictyostelium myosin phosphorylation are due to changes in myosin localization and increases in kinase activity.趋化因子引发的盘基网柄菌肌球蛋白磷酸化增加是由于肌球蛋白定位的变化和激酶活性的增加。
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Identification of two phosphorylated threonines in the tail region of Dictyostelium myosin II.盘基网柄菌肌球蛋白II尾部区域中两个磷酸化苏氨酸的鉴定。
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Effects of cytoplasmic acidification on clathrin lattice morphology.细胞质酸化对网格蛋白晶格形态的影响。
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盘基网柄菌中轻酶解肌球蛋白的表达会阻断正常的肌球蛋白II功能。

Expression of light meromyosin in Dictyostelium blocks normal myosin II function.

作者信息

Burns C G, Reedy M, Heuser J, De Lozanne A

机构信息

Department of Cell Biology, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

J Cell Biol. 1995 Aug;130(3):605-12. doi: 10.1083/jcb.130.3.605.

DOI:10.1083/jcb.130.3.605
PMID:7622561
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2120531/
Abstract

The ability of myosin II to form filaments is essential for its function in vivo. This property of self association is localized in the light meromyosin (LMM) region of the myosin II molecules. To explore this property in more detail within the context of living cells, we expressed the LMM portion of the Dictyostelium myosin II heavy chain gene in wild-type Dictyostelium cells. We found that the LMM protein was expressed at high levels and that it folded properly into alpha-helical coiled-coiled molecules. The expressed LMM formed large cytoplasmic inclusions composed of entangled short filaments surrounded by networks of long tubular structures. Importantly, these abnormal structures sequestered the cell's native myosin II, completely removing it from its normal cytoplasmic distribution. As a result the cells expressing LMM displayed a myosin-null phenotype: they failed to undergo cytokinesis and became multinucleate, failed to form caps after treatment with Con A, and failed to complete their normal developmental cycle. Thus, expression of the LMM fragment in Dictyostelium completely abrogates myosin II function in vivo. The dominant-negative character of this phenotype holds promise as a general method to disrupt myosin II function in many cell types without the necessity of gene targeting.

摘要

肌球蛋白II形成细丝的能力对其在体内的功能至关重要。这种自我缔合特性定位于肌球蛋白II分子的轻酶解肌球蛋白(LMM)区域。为了在活细胞背景下更详细地探究这一特性,我们在野生型盘基网柄菌细胞中表达了盘基网柄菌肌球蛋白II重链基因的LMM部分。我们发现LMM蛋白大量表达,并且正确折叠成α-螺旋卷曲螺旋分子。表达的LMM形成了大的细胞质内含物,由缠绕的短丝组成,周围是长管状结构网络。重要的是,这些异常结构隔离了细胞内天然的肌球蛋白II,使其完全脱离正常的细胞质分布。结果,表达LMM的细胞表现出肌球蛋白缺失表型:它们无法进行胞质分裂并变成多核细胞,用刀豆球蛋白A处理后无法形成帽,也无法完成正常的发育周期。因此,在盘基网柄菌中表达LMM片段完全消除了肌球蛋白II在体内的功能。这种表型的显性负性特征有望成为一种在许多细胞类型中破坏肌球蛋白II功能的通用方法,而无需进行基因靶向操作。