鳜碱性肌球蛋白轻链基因cDNA的克隆及其发育表达分析

肌球蛋白轻链是构成鱼类肌纤维主要组成部分,在鱼类肌肉生长和收缩过程中具有重要作用。鳜鱼具有生长快、肉质细嫩、味道鲜美、营养成分高等优良的性状。研究通过构建鳜肌肉组织cDNA文库分离到两个碱性肌球蛋白轻链基因,即MLC1和MLC3基因。序列分析显示MLC1和MLC3基因cDNA序列全长分别为1237bp和1070bp,分别编码192和150个氨基酸,除去MLC1N端多出的42个氨基酸残基,MLC1与MLC3氨基酸序列同源性为80.3%。通过PROSITEtools软件预测显示两种轻链都具有两个保守的EF-手相结构,其中第二个EF-hand结构除前三个氨基酸外同源性达100%。鱼类MLC3轻链N端没有高等脊椎动物MLC3特有标志序列。采用实时荧光定量PCR方法对鳜鱼MLC1和MLC3发育性表达分析表明,在原肠期开始有低量表达,与原肠期、尾芽期和肌肉效应期相比,心搏期和仔鱼期MLC1和MLC3表达量显著升高。研究结果首次提供了鳜肌肉组织肌球蛋白主要结构基因的分子生物学信息以及它们在鳜肌肉组织发生和功能的相关性。       

斑鳜肌球蛋白轻链2基因cDNA的克隆及其纵向表达分析

从斑鳜(Siniperca scherzeri)背部白色肌肉组织中提取总RNA,利用RT-PCR法克隆到斑鳜肌球蛋白轻链2基因(MLC2)(GenBank:GQ283000).斑鳜MLC2基因cDNA序列的开放阅读框的长度为513 bp,编码170个氨基酸,理论相对分子质量为19 105.61 Da,等电点为4.73.该开放阅读框具有4个EF-手相结构.斑鳜MLC2推导的氨基酸序列与已报道的其它6种鱼类MLC2氨基酸序列同源性在89%以上,其中与Ca2+结合的区域非常保守,氨基酸序列同源性为100%.用实时荧光定量PCR对斑鳜MLC2纵向表达分析显示,MLC2在斑鳜背肌的前部、中部和后部都有表达,但无显著差异.     

桔小实蝇V-ATPase G亚基基因的克隆及组织表达特异性分析

空泡型ATP酶（vacuolar-type H⁺-ATPase, V-ATPase）作为质子泵几乎在所有的真核生物细胞中发挥重要作用。本研究利用RT-PCR和RACE技术获得了桔小实蝇Bactrocera dorsalis (Hendel)V-ATPase G亚基序列全长, 命名为BdorATPG。测序结果表明, BdorATPG阅读框全长354 bp, 编码117个氨基酸。氨基酸序列比对表明, BdorATPG的N端序列与其他物种的ATPG亚基对应区域具有较高的序列一致性。BdorATPG与拟暗果蝇Drosophila pseudoobscura ATPG亚基的氨基酸序列一致性最高, 为88.9%。三维结构模建结果表明, BdorATPG N端（第1~59位氨基酸）序列为α-螺旋结构, 亲水性和疏水性氨基酸在螺旋两侧呈对称分布。BdorATPG在不同组织中的荧光定量PCR分析表明, BdorATPG在各组织中都有表达, 其中在触角中的表达量最高; 在雄虫生殖节中的表达量是雌虫中的6.04倍。结果提示BdorATPG可能在雄虫生殖生理过程中发挥重要作用。     

瓜实蝇嗅觉受体基因的克隆及表达谱分析

昆虫的嗅觉受体是一个高度变异的蛋白家族, 其中一类Or83b嗅觉受体在不同昆虫体内高度保守, 在昆虫的行为调控过程中起到十分重要的作用。为进一步探讨Or83b受体的功能, 本研究利用RT-PCR和RACE方法克隆获得瓜实蝇Bactrocera cucurbitae (Coquillett) Or83b-like受体的全长cDNA序列, 命名为BcucOr83b-like（GenBank登录号： HM745934）。测序结果表明, BcucOr83b-like开放阅读框全长1 422 bp,编码473个氨基酸残基。氨基酸序列比对表明, 此序列具有Or83b受体的典型特征, 序列中具有7个跨膜区和高度保守的C端区域。BcucOr83b-like与其他昆虫的Or83b具有较高的氨基酸序列一致性, 其中与桔小实蝇Bactrocera dorsalis（Hendel）Or83b的序列一致性高达99.6%。对该基因在瓜实蝇成虫不同组织和发育时期表达量的荧光定量PCR分析表明, BcucOr83b-like主要在瓜实蝇成虫触角中表达, 头部（去除触角）、 雌虫前足和翅中也有较高的表达; 瓜实蝇在各个发育时期的表达水平不同, 在刚羽化雌成虫中的表达量最高。本研究为深入研究瓜实蝇Or83b受体的功能提供了理论依据。     

翘嘴鳜肌球蛋白轻链3b基因(MLC3b)的分子克隆和特征分析

翘嘴鳜以其优良肉质性状近期已成为中国极具商品价值和大力推广的人工养殖名贵鱼类之一。为了解其控制优良肉质性状的遗传基础,本文采用同源克隆RT-PCR方法,获得该鱼肌球蛋白轻链MLC3b基因cDNA序列,该基因cDNA序列为453bp,编码150个氨基酸残基,通过PROSITE tools软件预测显示,该轻链具有两个保守的EF-手相结构和一个C-末端保守序列,且该MLC3轻链N端没有高等脊椎动物特有标志序列。MLC3b基因cDNA序列与MLC3a编码区的同源性达97.7%。本研究结果将为名贵鱼类肉质结构基因及功能的研究提供分子生物学基础。     

苜蓿体内H2S信号与Ca2+调节气孔运动的作用机制

为探究H₂S信号在苜蓿（Medicago sativa）体内调节气孔运动的作用,及在此过程中H₂S与Ca²⁺的关系,以蒺藜苜蓿（Medicago truncatula）的野生型和钙离子转运体突变体为试验材料,分别从转录水平、细胞水平和生理水平开展研究。采用qRT-PCR比较相关基因的表达量变化、荧光探针显示体内Ca²⁺含量、电极法测定H₂S含量、光学显微镜观察和测量气孔孔径等。结果表明：蒺藜苜蓿突变体NF3011和NF2734体内H₂S的含量与野生型相比极显著降低（P<0.01）;H₂S信号在一定程度上抑制钙离子转运体编码基因MTR_6g027580的表达;外源生理浓度H₂S熏蒸可诱导蒺藜苜蓿气孔关闭,与Ca²⁺通道阻断剂LaCl₃联合处理对野生型气孔运动未产生影响,而在突变体中的结果截然相反;利用荧光探针测定保卫细胞内的Ca²⁺含量,所得结果与气孔孔径的变化规律完全一致。综上所述,H₂S信号促进叶片保卫细胞内Ca²⁺的含量增加,最终表现为植物气孔孔径变小,在此过程中胞内Ca²⁺含量变化主要通过Ca²⁺转运体进行,少部分依赖Ca²⁺离子通道。该研究结果不仅在理论上丰富了H₂S信号的作用机制,更具应用于苜蓿生产实践并推广于其他作物的潜力。     

桔小实蝇肽聚糖识别蛋白基因BdPGRP-SB1的克隆及功能鉴定

【目的】为探究肽聚糖识别蛋白(PGRP)基因BdPGRP-SB1在桔小实蝇Bactrocera dorsalis免疫中的作用。【方法】本研究利用PCR克隆桔小实蝇BdPGRP-SB1全长cDNA序列;利用生物信息学软件对该基因核苷酸序列及其编码的氨基酸序列特征进行分析。采用RT-qPCR分析BdPGRP-SB1在桔小实蝇不同发育阶段(卵、幼虫、蛹、成虫)及5日龄成虫不同组织(中肠、马氏管、后肠、脂肪体、卵巢和精巢)中的表达模式;对桔小实蝇5日龄雌成虫分别注射大肠杆菌Escherichia coli 0111:B4肽聚糖(PGN-EB)和金黄色葡萄球菌Staphylococcus aureus肽聚糖(PGN-SA)后检测BdPGRP-SB1表达水平变化。利用RNAi沉默BdPGRP-SB1的表达,测定大肠杆菌和金黄色葡萄球菌诱导后桔小实蝇雌成虫的死亡率及大肠杆菌诱导后抗菌肽(AMP)基因attacin-A, defensin和diptercin表达变化情况。【结果】克隆获得桔小实蝇BdPGRP-SB1的全长cDNA序列(GenBank登录号: MN892482),开放阅读框长558 bp,编码185个氨基酸,其编码蛋白预测分子量为21.45 kD,等电点为8.57。序列分析表明,BdPGRP-SB1无跨膜结构域,具有PGRP保守结构域,前端具有信号肽,为分泌型蛋白;具有Zn²⁺依赖性酰胺酶活性和DAP型肽聚糖识别位点。系统进化分析发现,BdPGRP-SB1与辣椒实蝇B. latifrons的PGRP-SB1亲缘关系最近,氨基酸序列一致性达96%。发育表达模式表明,BdPGRP-SB1在桔小实蝇3日龄幼虫和成虫期高表达;组织表达谱结果显示BdPGRP-SB1在5日龄成虫各组织中均有表达,在脂肪体内表达量最高。PGN-EB和PGN-SA均能诱导桔小实蝇雌成虫体内BdPGRP-SB1表达水平变化。通过RNAi抑制BdPGRP-SB1表达后,注射大肠杆菌导致桔小实蝇雌成虫死亡率显著升高,以及attacin-A, defensin和diptercin表达量显著上调。【结论】结果说明桔小实蝇BdPGRP-SB1参与识别革兰氏阴性细菌,并可能参与桔小实蝇Imd途径调控其免疫反应。     

川芎嗪对模拟失重大鼠颈动脉平滑肌Ca2+敏感性的影响

目的：探讨川芎嗪对模拟失重大鼠颈动脉平滑肌收缩蛋白Ca²⁺敏感性的影响及机制。方法：21只雌性SD大鼠分为对照组（CON）、模拟失重组（TS）、模拟失重+川芎嗪灌饲组（LTZ）（n=7）。4周后测定大鼠颈动脉收缩性、收缩蛋白Ca²⁺敏感性及肌球蛋白轻链激酶抑制剂ML-7对以上指标的影响。结果：TS组苯肾上腺素（PHE）收缩力比CON组高25.14%（P<0.01）,LTZ组较TS组低13.46%（P<0.01）,较CON组高8.30%;ML-7可使CON、TS、LTZ组PHE收缩力分别降低8.84%、16.24%（P<0.01）和3.40%;TS组KCl收缩力比CON组高40.46%（P<0.01）,LTZ组较TS组低18.80%,较CON组高14.05%;ML-7可使CON、TS、LTZ组KCl收缩力分别降低21.97%（P<0.05）、21.88%（P<0.01）和10.84%;TS组pD2[Ca²⁺]比CON组高10.03%（P<0.01）,LTZ组较TS组低7.01%（P<0.01）,较CON组高2.32%;ML-7可使CON、TS、LTZ组pD2[Ca²⁺]分别降低2.42%、7.43%（P<0.01）和2.51%。结论：模拟失重大鼠颈动脉收缩增强可能是由动脉平滑肌收缩蛋白Ca²⁺敏感性增强所导致的。川芎嗪可改善模拟失重大鼠颈动脉的收缩功能,其机制可能与抑制血管平滑肌肌球蛋白轻链激酶继而降低Ca²⁺敏感性有关。     

镁转运体MGT7参与拟南芥对高钙环境的适应

高Ca²⁺环境对许多植物的生长不利, 因此研究植物对高Ca²⁺环境的适应机制非常重要。研究发现, 拟南芥(Ara- bidopsis thaliana)镁转运体MGT7功能缺失突变体mgt7-1和mgt7-2具有高Ca²⁺敏感表型: 在高Ca²⁺培养基上, 相对于野生型Col-0, 突变体叶鲜重显著下降, 但根长无显著差异。高Ca²⁺对MGT7启动子活性和包括MGT7在内的镁转运体基因表达无显著调节作用。Col-0与mgt7突变体之间, 在外加Ca²⁺诱导细胞质Ca²⁺瞬时升高和Ca²⁺含量方面无显著差异; 但是, 在正常和高Ca²⁺培养基上, mgt7突变体的Mg含量均显著低于Col-0。高Ca²⁺显著抑制Col-0和mgt7突变体内Mg的积累。因此我们假设, mgt7突变体的高Ca²⁺敏感表型是由于其体内Mg含量下降导致的。进一步的研究证实, 只有增加培养基中Mg²⁺的含量, 而不是N、P、K和S, 才可以使突变体的高Ca²⁺敏感表型得到恢复。     

转基因小鼠中外源基因部分内含子序列的缺失及其对转录的影响

利用PCR扩增及PCR测序在显微注射法产生的转基因小鼠中发现,整合在小鼠染色体上的肌球蛋白轻链2启动子(myosinlightchain2promoter,MLC2)-糜酶(chymase)外源融合基因存在两种形式,一种为全长的融合基因,另一种在糜酶结构基因的第一内含子中缺失了213bp的序列。RT-PCR结果表明,缺失了部分内含子序列的外源融合基因不能在转基因小鼠心脏中表达.而全长的外源融合基因则能较高水平地表达,竞争性PCR定量实验表明在200ng心脏总RNA反转录产物中约含5.05(±1.38)×106个糜酶cDNA分子。上述结果表明,糜酶结构基因的第一内含子可能对MLC2-糜酶基因的表达具有调控作用。     

Molecular cloning and expression analysis of a myosin light chain 1 (MLC‐1) gene from Indian meal moth Plodia interpunctella (Lepidoptera: Pyralidae)

Myosin light chain 1 (MLC‐1) protein acts in the organization, dynamics and transport processes associated with the cytoskeleton. In this work, an MLC‐1 gene was cloned and characterized from the Indian meal moth, Plodia interpunctella (Lepidoptera: Pyralidae). The isolated PiMLC‐1 cDNA is 913 bp, including a 5′‐untranslated region (UTR) of 79 bp, 3′‐UTR of 381 bp and an open reading frame (ORF) of 453 bp encoding a polypeptide of 150 amino acids, which contains two calcium binding domains (EF‐hands). The deduced PiMLC‐1 protein sequence has 39–94% comparison with other individuals. The qPCR analysis revealed that PiMLC‐1 was expressed in the four developmental stages (egg, larva, pupa and adult) and in all tissues tested, suggesting that it plays an important role in development of P. interpunctella. Based on the MLC‐1 amino acids, phylogenetic analysis showed a similar topology with the traditional classification, suggesting the potential value of the MLC‐1 protein in phylogenetic inference.     

Gene duplication and conversion events shaped three homologous, differentially expressed myosin regulatory light chain (MLC2) genes

Myosin II is a hexameric protein complex consisting of two myosin heavy chains, two myosin essential light chains and two myosin regulatory light chains. Multiple subunit isoforms exist, allowing great diversity in myosin II composition which likely impacts on its contractile properties. Little is known about the evolutionary origin, expression pattern and function of myosin regulatory light chain (MLC2) isoforms. We analysed the evolutionary relationship between smooth muscle (sm), nonmuscle (nm) and nonmuscle-like (nml) MLC2 genes, which encode three homologous proteins expressed in nonmuscle cells. The three genes arose by successive gene duplication events. The high sequence similarity between the tandemly arranged nm- and nml-MLC2 genes is best explained by gene conversion. Urea/glycerol-polyacrylamide gel electrophoresis and RNA analysis were employed to monitor expression of sm-, nm- and nml-MLC2 in human and mouse cell lines. Conspicuous differences between transformed and non-transformed cells were observed, with sm-MLC2 being suppressed in Ras-transformed cells. Our findings shed light on the evolutionary history of three homologous MLC2 proteins and point to isoform-specific cell growth-related roles in nonmuscle cell myosin II contractility.     

Wnt3a诱导小鼠胚胎干细胞向心肌细胞分化的研究

目的：研究Wnt3a在诱导小鼠胚胎干细胞心肌细胞分化中的作用和原理。方法：设计不同浓度,不同成分的Wnt3a条件培养基对小鼠胚胎干细胞诱导分化,对分化细胞进行形态学鉴定,通过免疫细胞化学检测心肌肌钙蛋白-T（cTnT）的表达,通过RT．PCR检测肌球蛋白重链（ot．MHC）和肌球蛋白轻链（MLC．2v）的表达。结果：Wnt3a诱导小鼠胚胎干细胞分化为心肌样细胞,分化细胞具有自动收缩性,免疫细胞化学检测心肌肌钙蛋白．T（cTllT）表达阳性,RT．PCR检测肌球蛋白重链（d—MHC）和肌球蛋白轻链（MLC-2v）表达阳性。经典Wnt信号途径的抑制剂Frizzled一8／Fc,能够抑制Wnt3a的诱导分化作用。结论：Wnt3a通过经典Wnt信号途径诱导小鼠胚胎干细胞向心肌细胞分化。     

Nerve-dependent accumulation of myosin light chain 3 in developing limb musculature

Myosin alkali light chain accumulation in developing quail limb musculature has been analysed on immunoblots using a monoclonal antibody which recognizes an epitope common to fast myosin light chain 1 (MLC1f) and fast myosin light chain 3 (MLC3f). The limb muscle of early embryos (i.e. up to day 10 in ovo) has a MLC profile similar to that observed in myotubes cultured in vitro; although MLC1f is abundant, MLC3f cannot be detected. MLC3f is first detected in 11-day embryos. To determine whether this alteration in MLC3f accumulation is nerve or hormone dependent, limb buds with and without neural tube were cultured as grafts on the chorioallantoic membrane of chick hosts. Although differentiated muscle develops in both aneural and innervated grafts, innervated grafts contain approximately three times as much myosin as aneural grafts. More significantly, although aneural grafts reproducibly accumulate normal levels of MLC1f, they fail to accumulate detectable levels of MLC3f. In contrast, innervated grafts accumulate both MLC1f and MLC3f, suggesting that the presence of neural tube in the graft promotes the maturation, as well as the growth, of muscle tissue. This is the first positive demonstration that innervation is necessary for the accumulation of MLC3f that occurs during normal limb development in vivo.     

Molecular cloning, sequence identification and expression analysis of novel caprine MYLPF gene

Skeletal muscle genes are important potentially functional candidate genes for livestock production and meat quality. Myosin regulatory light chain (MLC) regulates myofilament activation via phosphorylation by Ca²⁺ dependent myosin light chain kinase. The cDNA of the myosin light chain, phosphorylatable, fast skeletal muscle (MYLPF) gene from the longissimus dorsi of Tianfu goat was cloned and sequenced. The results showed that MYLPF full-length coding sequence consists of 513 bp and encodes 170 amino acids with a molecular mass of 19.0 kD. Two EF-hand superfamily domain of MYLPF gene conserved between caprine and other animals. The deduced amino acid sequence of MYLPF shared significant identity with the MYLPF from other mammals. A phylogenetic tree analysis revealed that the caprine MYLPF protein has a close genetic relationship and evolutional distance with MYLPF in other mammals. Analysis by RT-PCR showed that the MYLPF mRNA was detected in heart, liver, spleen, lung, kidney, gastrocnemius, abdominal muscle and longissimus dorsi. In particular, high expression levels of MYLPF mRNA were detected in the longissimus dorsi, gastrocnemius and abdominal muscle, and low level of expressions were observed in liver, spleen, lung and kidney. In addition, the temporal expression analysis further showed MYLPF expression decreased gradually with age in the skeletal muscle. This may be important as muscle growth occurs mainly in young age in goats. Western blotting results detected the MYLPF protein in four of the tissues in which MYLPF was shown to be expressed; the four exceptions were liver, spleen, lung and kidney.     

Characterization and ontogenetic expression analysis of the myosin light chains from the fast white muscle of mandarin fish Siniperca chuatsi

Three full-length complementary DNA (cDNA) clones were isolated encoding the skeletal myosin light chain 1 (MLC1; 1237 bp), myosin light chain 2 (MLC2; 1206 bp) and myosin light chain 3 (MLC3; 1079 bp) from the fast white muscle cDNA library of mandarin fish Siniperca chuatsi. The sequence analysis indicated that MLC1 and MLC3 were not produced from differentially spliced messenger RNAs (mRNA) as reported in birds and rodents but were encoded by different genes. The MLC2 encodes 170 amino acids, which include four EF-hand (helix-loop-helix) structures. The primary structures of the Ca(2+)-binding domain were well conserved among the MLC2s of seven other fish species. The ontogenetic expression analysis by real-time PCR showed that the three light-chain mRNAs were first detected in the gastrula stage, and their expression increased from the tail bud stage to the larval stage. All three MLC mRNAs showed longitudinal expression variation in the fast white muscle of S. chuatsi, especially MLC1 which was highly expressed at the posterior area. Taken together, the study provides a better understanding about the MLC gene structure and their expression pattern in muscle development of S. chuatsi.     

Expression of cardiac myosin light chain 2 during embryonic heart development in medaka fish,Oryzias latipes,and phylogenetic relationship with other myosin light chains

Cardiac myosin light chain 2 (MLC‐2) plays a key role in heart development, contraction, and embryo and adult heart maintenance. In some animals, defects in the function of cardiac MLC‐2 cause hypertrophic cardiomyopathy. To illuminate the functions of cardiac MLC‐2 in embryonic heart formation and contraction, and into the evolution of MLC‐2, we characterized the expression and requirement for medaka cardiac MLC‐2 gene in the developing heart. Medaka cardiac MLC‐2 cDNA (mcmlc2) was isolated and its gene expression pattern was determined. The mcmlc2 was found to be expressed in the bilateral cardiac mesoderm, the formed heart tube, and in both the differentiated ventricle and atrium. Knockdown of mcmlc2 function caused severe cardiac disorders, including edema in the atrium and sinus venosus. Using phylogenetic analysis, we found that physiological variations in the MLC‐2 molecules evolved due to amino acid changes in the Ca²⁺ binding domain during molecular evolution. Our findings concerning the function and expression of mcmlc2 are nearly identical with those of other MLC‐2 genes, and our phylogenetic analysis suggests that during evolution, the variations in physiological function within the MLC‐2 gene family have arisen from a change in the amino acids in the Ca²⁺ binding domain in the MLC‐2 molecule.     

Location of the inhibitory region of smooth muscle myosin light chain kinase

Proteolysis by trypsin of gizzard myosin light chain kinase (MLC kinase) in the absence of Ca2+-calmodulin produced a 64,000-dalton inactive fragment which was converted to a 61,000-dalton Ca2+-calmodulin-independent active fragment. This confirmed previous results (Ikebe, M., Stepinska, M., Kemp, B. E., Means, A. R., and Hartshorne, D. J. (1987) J. Biol. Chem. 262, 13828-13834). On the other hand, proteolysis of MLC kinase in the presence of Ca2+-calmodulin initially produced a 66,000-dalton Ca2+-calmodulin-dependent active fragment which was converted to a 61,000-dalton Ca2+-calmodulin-independent active fragment with further proteolysis. The amino acid sequences from the N terminus of the 66,000-dalton, 64,000-dalton, and 61,000-dalton fragments were determined. The sequence was not found in the reported partial amino acid sequence of MLC kinase (C-terminal 60% of whole sequence) (Guerriero, V., Jr., Russo, M. A., Olson, N. J., Putkey, J. A., and Means, A. R. (1986) Biochemistry 25, 8372-8381), and, therefore, the cleavage sites are in the remaining 40% N-terminal portion of the sequence of MLC kinase. The C terminus of these MLC kinase fragments was determined by employing the carboxypeptidases A, B, and Y digestion followed by the amino acid analysis of the released amino acids. As a result, it was concluded that the C terminus of the 66,000-dalton, 64,000-dalton, and 61,000-dalton MLC kinase fragments are arginine 522, lysine 490 and arginine 494, and lysine 473, respectively. These results show that the inhibitory domain is in the amino acid sequence of 474-490, and that the amino acid sequence 494-522 confers the calmodulin-dependent kinase activity.     

An increase or a decrease in myosin II phosphorylation inhibits macrophage motility

Myosin II purified from mammalian non-muscle cells is phosphorylated on the 20-kD light chain subunit (MLC20) by the Ca2+/calmodulin-dependent enzyme myosin light chain kinase (MLCK). The importance of MLC20 phosphorylation in regulating cell motility was investigated by introducing either antibodies to MLCK (MK-Ab) or a Ca2+/calmodulin-independent, constitutively active form of MLCK (MK-) into macrophages. The effects of these proteins on cell motility were then determined using a quantitative chemotaxis assay. Chemotaxis is significantly diminished in macrophages containing MK-Ab compared to macrophages containing control antibodies. Moreover, there is an inverse relationship between the number of cells that migrate and the amount of MK-Ab introduced into cells. Interestingly, there is also an inverse relationship between the number of cells that migrate and the amount of MK- introduced into cells. Other experiments demonstrated that MK-Ab decreased intracellular MLC20 phosphorylation while MK- increased MLC20 phosphorylation. MK- also increased the amount of myosin associated with the cytoskeleton. These data demonstrate that the regulation of MLCK is an important aspect of cell motility and suggest that MLC20 phosphorylation must be maintained within narrow limits during translational motility by mammalian cells.