雷州黑鸭胚胎期骨骼肌发育表达与功能分析

为保护雷州黑鸭优异的肉用性能,并开发利用这一珍贵的种质资源,研究选取雷州黑鸭为实验素材,对其胚胎期胸腿肌进行组织切片观察,并采用q RT-PCR与Western blot试验方法检测了Pax3、DCN和MSTN等基因在8、13、18、23和28胚龄胸腿肌中的发育性表达规律。同时用q RT-PCR法检测了雷州黑鸭28胚龄时Pax3、DCN和MSTN基因在各组织中m RNA的差异性表达量。胸腿肌组织切片观察雷州黑鸭胚胎期腿肌的发育明显早于胸肌;荧光定量PCR结果显示,雷州黑鸭Pax3、DCN和MSTN基因在各阶段胸腿肌中的相对表达量在23和28胚龄期最高,显著高于其它胚龄(P0.05);雷州黑鸭28胚龄时各组织中Pax3、DCN和MSTN基因在胸肌和腿肌中的表达显著高于其他组织(P0.05);Western blot结果表明,在胸腿肌中Pax3、DCN和MSTN蛋白的表达量在8胚龄期最低,在23胚龄时表达量显著高于其它胚龄(P0.05),达到高峰。结合切片图对比表达模式的分析表明在肌纤维的形成以及生长发育过程中,Pax3、DCN和MSTN基因对骨骼肌的生理特性起到决定性作用,在雷州黑鸭胚胎期骨骼肌发育过程中的不同阶段调控着早期胚胎中前体肌细胞的分化、增殖、促进肌纤维的形成。     

鳜慢肌胚后发育与生长特征

鱼类快肌和慢肌分别占据骨骼肌的不同位置,表现不同的生长发育特征。为了解鳜(Sinipercachuatsi)慢肌纤维的胚后发育特征,本研究通过制作孵化后1～33日龄鳜个体的石蜡切片,采用慢肌特异抗体的免疫组织化学染色,观察了背鳍起点处躯干横切面慢肌的发育变化特征,并利用图像分析软件统计慢肌纤维的数目和面积。结果表明,孵化后鳜仔鱼慢肌位于水平肌隔附近,呈楔形,向背、腹两侧生长。孵化后1～9日龄为单层肌纤维,11日龄发育为多层肌纤维,19日龄覆盖侧线附近,33日龄延伸至背侧第2背肌节、腹侧腹部肌肉2/3处,并在水平肌隔和侧线处分别形成两个肌群。位于骨骼肌最外层的扁平状表层细胞,可能为慢肌增生生长的主要来源。躯干单侧慢肌肌纤维数目由孵化后6个增加至315个,总面积从13.18μm2增加到7 839.58μm2,孵化后13日龄的增生生长占优势,其他发育阶段,肥大生长一直占主导优势。     

心室肌的大体与显微的层次解剖研究

目的:通过对心室肌的大体解剖与组织学切片显示心室肌纤维的层次走向,比较心肌传统概念与心肌带理论的差异.方法:(1)应用大体解剖、组织切片HE染色、虚拟切片扫描方法显示心室肌的纤维走向及层次构造.(2)将防腐固定后的成人正常心脏顺心肌纤维方向分层解剖心肌,使之展开成带,验证心肌带理论.结果:将防腐固定的成人正常心脏经改良的解剖方法解剖,可解剖出一条完整的心肌带,分为2个环,4个段.心肌带呈螺旋走向.用大体解剖与组织切片HE染色、虚拟切片扫描显示右心室肌起始于纤维三角为一条单层肌肉带,左心室肌分为三层肌纤维起始于纤维三角与纤维环,肌纤维从纤维三角与纤维环持续由外向内转变呈现为一种交错结构,纵行的浅层心肌纤维在心尖以90°的角返回心底方向,构成深层心室肌形成肉柱,部分心肌纤维斜、横行构成中层心室肌.三者在心尖呈现出一种螺旋形结构.应用虚拟切片扫描技术能完整、清楚地显示心室肌某一切面的结构走向.结论:心肌传统理论与心肌带理论并未完全冲突,心肌带理论的降段、左室断、升段与传统理论的浅、中、深三层相对应.     

骨骼肌卫星细胞对肉品质的影响及其分化调控

骨骼肌卫星细胞是一种肌源性干细胞, 在骨骼肌的生长、发育及肌肉损伤修复中有着至关重要的作用。肌卫星细胞通过增殖、分化融合肌纤维形成新的肌核从而导致骨骼肌纤维的肥大以及骨骼肌纤维类型的相互转化, 进而影响肉品质的形成。文章从肌纤维的发育与肉品质形成、卫星细胞分化与肌纤维特征的相关性等方面, 对卫星细胞的Notch等经典遗传信号通路和miRNA等表观遗传调控及其对肉品质的影响进行了综述。     

小鼠胚胎心流出道发育中胰岛因子1的表达及意义

目的观察胰岛因子1(Islet-1,ISL-1)在小鼠胚胎心流出道发育中的表达,探讨ISL-1阳性细胞在第二生心区的时空分布特点及其在心流出道发育中的作用。方法 15只胚龄8.5d~12d小鼠胚胎心连续石蜡切片,选用抗α-平滑肌肌动蛋白(α-smooth muscle actin,α-SMA)、抗心肌肌球蛋白重链(myosinheavy chain,MHC)和抗ISL-1抗体,进行免疫组织化学染色。结果胚龄8.5d~10d,ISL-1阳性细胞相继出现在流出道远端、心包腔背侧脏壁和体壁中胚层、原始咽腹外侧间充质及第2对鳃弓核心间充质,并逐渐分化为心肌细胞添加到流出道远端;胚龄11d,咽腹侧ISL-1阳性细胞形成独特的锥形结构,形成主肺动脉隔的雏形;胚龄12d,ISL-1阳性锥形结构与流出道远端心内膜垫融合形成主肺动脉隔,此时ISL-1阳性细胞开始分化为平滑肌细胞,参与心包腔内升主动脉、肺动脉干和主肺动脉隔的发育。结论第二生心区涵盖了原始咽腹外侧间充质、心包腔背侧壁中胚层及鳃弓核心间充质等多个区域,其中的ISL-1阳性细胞具有多向分化潜能,在心发育的不同阶段可以分化为不同类型的细胞,参与流出道的正常发育。     

肌细胞增强因子2在心力衰竭过程中的作用

心脏在长期过量负荷及神经体液系统过度激活的影响下,可发生以心肌细胞肥大、心肌纤维排列紊乱、心肌间质细胞增生及胚胎基因再表达增加为主的病理改变,从而引起心脏泵功能减退、心室扩张、心室肥厚和纤维化,最终导致心力衰竭.肌细胞增强因子2(myocyte enhancerfactor 2,MEF2)是一种特定的转录因子,其主要功能是促进肌细胞分化过程中的基因转录,在骨骼肌、心肌、平滑肌的发育过程中起介导细胞分化的作用.近年来的研究发现,在心力衰竭过程中.MEF2提供了心室重构信号转导过程中的作用靶点,可能参与了心室肥厚与心力衰竭的过程.     

外胚间充质干细胞构建组织工程骨骼肌的应用研究

目的:探讨利用大鼠颌突外胚间充质干细胞构建组织工程骨骼肌的可行性,并观察对骨骼肌缺损的修复重建的促进效应。方法:取妊娠E 11.5胎鼠颌突外胚间充质干细胞,纯化后在含5ml/L体积浓度二甲基亚砜的DMEM/F12培养基中诱导分化为骨骼肌样细胞,将细胞种植于BAM膜上培养形成组织工程骨骼肌。将其移植入大鼠骨骼肌缺损模型,手术后14 d观察骨骼肌恢复情况,同期进行组织学及免疫组化染色鉴定。结果:经诱导后外胚间充质干细胞可向骨骼肌样细胞转化,构建的组织工程骨骼肌可加速缺损的修复重建,组织学染色显示外胚间充质干细胞具有正常骨骼肌的组织形态,可表达成肌相关蛋白MyOD。结论:诱导后的外胚间充质干细胞可作为种子细胞构建组织工程骨骼肌,本实验为临床肌肉的缺损修复奠定了理论基础。     

MicroRNA调控哺乳动物骨骼肌发育

MicroRNA (miRNA)是一类长度大约为22 bp的小分子非编码RNA,广泛存在于哺乳动物中,部分miRNA表达具有时空和组织特异性。哺乳动物中miRNA主要通过与靶基因3° UTR区结合抑制其翻译,调控机体生物学功能。miRNA在哺乳动物骨骼肌发育中发挥重要调节作用。哺乳动物骨骼肌发育是一个复杂的生物学过程,包括骨骼肌干细胞增殖、迁移、分化,成肌细胞增殖、分化、肌管融合,肌纤维肥大,能量代谢,纤维类型转换等。miRNA参与骨骼肌发育的各个环节,通过靶向各个时期的关键因子调控骨骼肌发育。本文对miRNA在骨骼肌发育中的调控作用进行了综述,以期为深入理解骨骼肌发育规律提供参考。     

去负荷小鼠比目鱼肌收缩特性和纤维类型转化

目的:探讨去负荷后小鼠比目鱼肌的收缩特性与骨骼肌纤维类型转化之间的关系。方法:采用离体肌肉灌流技术和电刺激方法,在小鼠后肢去负荷28 d引起骨骼肌萎缩后,观察比目鱼肌单收缩、强直收缩能力和肌疲劳指标等收缩特性的改变,同时利用组织免疫荧光染色和实时定量聚合酶链式反应(real-time PCR)等技术检测去负荷后比目鱼肌快慢肌纤维组成和纤维类型转化的变化。结果:去负荷28 d后,小鼠比目鱼肌单收缩力、强直收缩能力和疲劳指数(fatigue index)均有显著性下降,同时伴有快肌纤维亚型的增加和慢肌纤维亚型的减少。结论:去负荷28 d后小鼠比目鱼肌收缩特性的改变和快慢肌纤维类型的转化有关。     

尾部悬吊对达乌尔黄鼠比目鱼肌形态及 mATP 酶活性的影响

采用尾部悬吊法建立后肢骨骼肌废用的动物模型,以肌球蛋白ATP酶(mATPase)法测定比目鱼肌的mATPase活性,依据mATPase染色结果进行肌纤维分型,并测量肌纤维横截面积(Cross-section area,CSA),首次观察了尾部悬吊对达乌尔黄鼠比目鱼肌湿重、CSA和梭外肌、梭内肌纤维mATPase活性的影响,并与尾部悬吊大鼠进行了比较。旨在探讨冬眠动物骨骼肌在废用状态下的变化。结果显示,尾部悬吊14d可使大鼠比目鱼肌湿重体重比下降35.52%(P<0.001),Ⅰ型肌纤维CSA和Ⅱ型肌纤维CSA分别下降18.91%和20.68%(P<0.05);肌纤维平均CSA减少20.45%(P<0.01)。比目鱼肌中Ⅰ型肌纤维的构成比由对照组的80.61%降低为66.83%,Ⅱ型肌纤维的构成比由19.39%增加到33.17%(P<0.001);梭内肌纤维mATPase活性增强,核袋1纤维的mATPase染色由阴性(-)转变为强阳性( ),核袋2纤维和核链纤维由阳性( )转变为强阳性( )。而达乌尔黄鼠在尾部悬吊14d后,比目鱼肌湿重仅比对照组下降0.05%,Ⅰ、Ⅱ型肌纤维CSA与平均CSA分别比对照组减少0.84%、0.63%和0.37%,均无明显差异(P>0.05);与对照组相比,比目鱼肌中Ⅰ型肌纤维的构成比从82.55%减少到77.30%,Ⅱ型肌纤维的构成比由17.45%增加到22.70%(P<0.05);梭内肌纤维mATPase活性亦明显升高,核袋1纤维的mATPase染色由对照组的阴性(-)转化为强阳性( ),核袋2纤维及核链纤维则由对照组的阳性( )转化为核袋2纤维呈阳性( ),核链纤维则呈弱阳性( )。结果表明:尾部悬吊可致大鼠比目鱼肌明显萎缩;达乌尔黄鼠比目鱼肌则无明显萎缩;两者比目鱼肌梭内、外肌mATPase活性均明显升高。     

卵泡抑素相关蛋白的病理生理功能

卵泡抑素相关蛋白(follistatin related protein,FRP)是一种细胞外基质糖蛋白,该蛋白参与细胞增殖、迁移、组织重塑、胚胎发育、细胞间相互作用及多种病理生理过程.近年研究显示,该蛋白同时具有抑制细胞凋亡和抑制细胞增殖的双重功能:在心肌缺血的动物模型中,FRP被证实有保护心肌细胞、抗凋亡、促进内皮细胞增殖等功能;FRP也可由血管平滑肌细胞合成分泌,并具有反馈调节平滑肌细胞功能的作用,该蛋白还可抑制多种肿瘤细胞增殖.     

Embryonic chicken skeletal, cardiac, and smooth muscles express a common embryo-specific myosin light chain

It has been demonstrated that embryonic chicken gizzard smooth muscle contains a unique embryonic myosin light chain of 23,000 mol wt, called L23 (Katoh, N., and S. Kubo, 1978, Biochem. Biophys. Acta, 535:401-411; Takano-Ohmuro, H., T. Obinata, T. Mikawa, and T. Masaki, 1983, J. Biochem. (Tokyo), 93:903-908). When we examined myosins in developing chicken ventricular and pectoralis muscles by two-dimensional gel electrophoresis, the myosin light chain (Le) that completely comigrates with L23 was detected in both striated muscles at early developmental stages. Two monoclonal antibodies, MT-53f and MT-185d, were applied to characterize the embryonic light chain Le of striated muscles. Both monoclonal antibodies were raised to fast skeletal muscle myosin light chains; the former antibody is specific to fast muscle myosin light chains 1 and 3, whereas the latter recognizes not only fast muscle myosin light chains but also the embryonic smooth muscle light chain L23. The immunoblots combined with both one- and two-dimensional gel electrophoresis showed that Le reacts with MT-185d but not with MT-53f. These results strongly indicate that Le is identical to L23 and that embryonic chicken skeletal, cardiac, and smooth muscles express a common embryo-specific myosin light chain.     

In ovo monitoring of smooth muscle fiber development in the chick embryo: diffusion tensor imaging with histologic correlation

Background

Magnetic resonance imaging is a noninvasive method of evaluating embryonic development. Magnetic resonance diffusion tensor imaging, which is based on the measuring the directional diffusivity of water molecules, is an established method of evaluating tissue structure. Prolonged imaging times have precluded the use of embryonic diffusion tensor imaging due to motion artifact. Using temperature-based motion suppression, we aimed to investigate whether diffusion tensor imaging can be used to monitor embryonic smooth muscle development in ovo, and to determine the correlation between histologically-derived muscle fiber fraction, day of incubation and diffusion tensor imaging fractional anisotropy values and length of tracked fibers.

Methodology/Principal Findings

From a set of 82 normally developing fertile chicken eggs, 5 eggs were randomly chosen each day from incubation days 5 to 18 and cooled using a dual-cooling technique prior to and during magnetic resonance imaging at 3.0 Tesla. Smooth muscle fibers of the gizzard were tracked using region of interests placed over the gizzard. Following imaging, the egg was cracked and the embryo was fixated and sectioned, and a micrograph most closely corresponding to the acquired magnetic resonance image was made. Smooth muscle fiber fraction was determined using an automated computer algorithm.

Conclusions/Significance

We show that diffusion tensor images of smooth muscle within the embryonic gizzard can be acquired in ovo from incubation day 11 through hatching. Length of tracked fibers and day of incubation were found to have statistical significance (p<0.05) by multiple linear regression correlation with histologic specimens of sacrificed embryos from day 11 of incubation through hatching. The morphologic pattern of development in our histologic specimens corresponds to the development of embryonic gizzard as reported in the literature. These results suggest that diffusion tensor imaging can provide a noninvasive method of evaluating in ovo development of smooth muscle tissue.     

Differences in the Developmental Fate of Cultured and Noncultured Myoblasts When Transplanted into Embryonic Limbs

Myoblasts from embryonic, fetal, and adult quail and chick muscles were transplanted into limb buds of chick embryos to determine if myoblasts can form muscle fibers in heterochronic limbs and to define the conditions that affect the ability of transplanted cells to populate newly developing limb musculature. Myoblasts from each developmental stage were either freshly isolated and transplanted or were cultured prior to transplantation into limb buds of 4- to 5-day (ED4-5) chick embryos. Transplanted myoblasts, regardless of the age of the donor from which they were derived, formed muscle fibers within embryonic limb muscles. Transplanted cloned myoblasts formed muscle fibers, although there was little evidence that the number of transplanted myoblasts significantly increased following transplantation or that they migrated any distance from the site of injection. The fibers that formed from transplanted clonal myoblasts often did not persist in the host limb muscles until ED10. Diminished fiber formation from myoblasts transplanted into host limbs was observed whether myoblasts were cloned or cultured at high density. However, when freshly isolated myoblasts were transplanted, the fibers they formed were numerous, widely dispersed within the limb musculature, and persisted in the muscles until at least ED10. These results indicate that transplanted myoblasts of embryonic, fetal, and adult origin are capable of forming fibers during early limb muscle formation. They also indicate that even in an embryonic chick limb where proliferation of endogenous myoblasts and muscle fiber formation is rapidly progressing, myoblasts that are cultured in vitro do not substantially contribute to long-term muscle fiber formation after they are transplanted into developing limbs. However, when the same myoblasts are freshly isolated and transplanted without prior cell culture, substantial numbers of fibers form and persist after transplantation into developing limbs. Thus, these studies demonstrate that the extent to which transplanted myoblasts fuse to form fibers which persist in host musculature depends upon whether donor myoblasts are freshly isolated or maintained in vitro prior to injection.     

CCN5 Expression in mammals. II. Adult rodent tissues

CCN5 is a secreted heparin- and estrogen-regulated matricellular protein that inhibits vertebrate smooth muscle cell proliferation and motility. CCN5 is expressed throughout murine embryonic development in most organs and tissues. However, after embryonic development is complete, we hypothesized that CCN5 distribution would be largely restricted to small set of tissues, including smooth muscle cells of the arteries, uterus, airway, and digestive tract. Because CCN5 inhibits proliferation of smooth muscle cells in vitro, it might function to prevent excessive growth in vivo. In contrast, another member of the CCN family, CCN2, promotes smooth muscle cell proliferation in vitro, and thus it was expected that its expression levels would be low in uninjured normal adult tissues. Frozen sections from adult tissues and organs were analyzed immunohistochemically using anti-CCN5 and anti-CCN2 antibodies. Both proteins were detected in arteries, the uterus, bronchioles, and the digestive tract as expected, and also in many other tissues including the pancreas, spleen, liver, skeletal muscle, ovary, testis, thymus, brain, olfactory epithelium, and kidney. CCN5 and CCN2 protein was found in smooth muscle, endothelial cells, epithelial cells, skeletal muscle, cells of the nervous system, and numerous other cell types. In many cells, both CCN5 and CCN2 was present in the nucleus. Rather than having opposite patterns of localization, CCN5 and CCN2 often had similar sites of expression. The wide distribution of both CCN5 and CCN2 suggests that both proteins have additional biological functions beyond those previously identified in specific cellular and pathological models.     

CCN5 expression in mammals

The six proteins of the CCN family have important roles in development, angiogenesis, cell motility, proliferation, and other fundamental cell processes. To date, CCN5 distribution in developing rodents and humans has not been mapped comprehensively. CCN5 strongly inhibits adult smooth muscle cell proliferation and motility. Its anti-proliferative action predicts that CCN5 would not be present in developing tissues until the proliferation phase of tissue morphogenesis is complete. However, estrogen induces CCN5 expression in epithelial and smooth muscle cells, suggesting that CCN5 might be widely expressed in embryonic tissues exposed to high levels of estrogen. 9–16 day murine embryos and fetuses and 3–7 month human fetal tissues were analyzed by immunohistochemistry. CCN5 was detected in nearly all developing tissues. CCN5 protein expression was initially present in most tissues, and at later times in development tissue-specific expression differences were observed. CCN5 expression was particularly strong in vascular tissues, cardiac muscle, bronchioles, myotendinous junctions, and intestinal smooth muscle and epithelium. CCN5 expression was initially absent in bone cartilaginous forms but was increasingly expressed during bone endochondral ossification. Widespread CCN5 mRNA expression was detected in GD14.5 mice. Although CCN2 and CCN5 protein expression patterns in some adult pathologic conditions are inversely expressed, this expression pattern was not found in developing mouse and human tissues. The widespread expression pattern of CCN5 in most embryonic and fetal tissues suggests a diverse range of functions for CCN5. Electronic supplementary material The online version of this article (doi:) contains supplementary material, which is available to authorized users.     

A chicken embryo-specific myosin light chain (L23) appears to be identical with one of brain myosin light chains

A novel embryo-specific myosin light chain of 23 kDa molecular weight (L23) was found previously in embryonic chicken skeletal, cardiac, and smooth muscles (Takano-Ohmuro et al. (1985) J. Cell Biol. 100, 2025-2030). When we examined myosin in embryonic and adult brain by two-dimensional electrophoresis, 23 kDa myosin light chain present in brain (Burridge & Bray (1975) J. Mol. Biol. 99, 1-14) comigrated with L23. Two monoclonal antibodies, EL-64 and MT-185d, were applied to clarify the identity of the brain 23 kDa myosin light chain and the chicken embryonic muscle L23. The two antibodies recognize different antigenic determinants in the L23 molecule; the former antibody is specific for L23, whereas the latter recognizes the sequence common to fast skeletal muscle myosin light chains 1 and 3, and also L23. The immunoblots combined with two-dimensional gel electrophoresis showed that both EL-64 and MT-185d can bind to the brain 23 kDa myosin light chain as well as the chicken embryonic muscle L23. These results indicate that chicken brain and chicken embryonic muscles contain a common myosin light chain of 23 kDa molecular weight.     

Expression of proto-oncogenes and muscle specific genes during cardiac hypertrophy and development in rats and humans

A regulatory interdependence of expression of proto-oncogenes and muscle specific genes observed in smooth muscle was examined in cardiac muscle during normal development and hypertrophy both in rats and humans. During normal development in rats, myosin light chain 2 expression is very low at prenatal stages, while c-fos expression starts from the early stages of embryonic development. In aorta constricted rats c-fos induction occurs within 30 min whereas myosin light chain 2 expression is sufficiently high only after 3 or 4 days of post operative period. In the case of humans, the expression of myosin light chain 2 as well as c-fos occurs at high levels during embryonic development. Similar results were obtained with tissue samples obtained from patients with cardiac abnormalities. Induction of the c-fos gene in cultured myocytes by 12-O-tetradeeanoylphorbol 13-acetate has no influence on the expression of myosin light chain 2. These studies were extended with studies on c-myc and Β-myosin heavy chain gene expression which revealed a similar pattern of expression as that of c-fos and myosin light chain 2. These results have indicated that the expression of proto-oncogenes in cardiac muscle may be independently regulated from the expression of muscle specific genes.     

Immunolocalization of basic fibroblast growth factor during chicken cardiac development

Basic fibroblast growth factor (bFGF) has been identified in cultured cardiac myocytes as well as in myocardial tissue of both embryonic and adult organisms; bFGF has also been demonstrated to regulate proliferation and differentiation of these cells in culture. Such studies suggest a possible role for bFGF in cardiac myogenesis. In vitro studies using cultured endothelial and neuronal cells also suggest that myocyte-derived bFGF may be involved in the regulation of vascularization and/or innervation of the developing heart. We have generated a spatial and temporal map for bFGF in the developing chick heart using immunohistochemical techniques and our monospecific polyclonal rabbit antihuman bFGF IgG. A progressive decrease in bFGF expression was seen in the highly trabeculated region of the ventricular myocardium, relative to the myocardium directly underlying the epicardial tissue, with increasing developmental age. bFGF expression was limited to the cytoplasm of cardiac myocytes; neither vascular endothelium nor smooth muscle contained anti-bFGF immunoreactive material. A correlation between the temporal and spatial pattern of bFGF expression seen here, with the pattern of myocyte proliferation and differentiation reported by others, suggests a role for bFGF in the autocrine regulation of myocyte proliferation and differentiation.