模拟微重力下秀丽隐杆线虫的力学感知和肌萎缩的发生机制——太空飞行线虫试验地面平行对照研究部分

目前,微重力导致肌萎缩的分子机制尚不清楚,重力感知是该事件发生的关键环节．为了回答这一问题,在此之前首先实施了太空线虫试验,这部分结果已经在本刊报道过．而本次研究主要是在地面上建立了模拟微重力环境,观察处理后秀丽隐杆线虫（C.elegans）体壁肌细胞结构和功能的变化,一方面用于验证太空试验,同时比较两种处理结果的异同,以便于评价地面模拟微重力的有效性．经过14天19．5h旋转模拟微重力处理后,对线虫生存率和运动能力进行了观察,并检测了几个重要的肌相关基因表达和蛋白质水平．模拟微重力下线虫生存率没有明显变化,但运动频率显著下降,爬行轨迹也发生了轻微改变,运动幅度降低,提示线虫运动功能出现障碍．从形态学上观察发现：肌球蛋白A（myosin A）免疫荧光染色显示模拟微重力组肌纤维面积缩小,而肌细胞致密体（dense-body）染色可见荧光亮度下降．这些结果直接提示模拟微重力使线虫出现了肌萎缩．随后Western blotting试验结果揭示,模拟微重力组线虫体壁肌的主要结构蛋白——myosin A含量减少,进一步确证了微重力性肌萎缩发生．在基因水平,旋转后抗肌萎缩蛋白基因（dys-1）表达明显上升,而hlh-1,unc-54,myo-3和egl-19的mRNA水平均下调,提示dys-1在骨骼肌感知和传导力学信息方面有重要作用,而hlh-1,unc-54,myo-3和egl-19则分别从结构和功能两个途径促进了微重力性肌萎缩的发生和发展．本次试验所得到的结果同太空飞行试验结果十分相似,一方面强化了太空试验结论,另一方面说明在地面上模拟微重力对生物体进行研究是有效可行的,将有助于提高太空试验的质量．     

空间环境对秀丽线虫行为及生长发育研究进展

与秀丽线虫有关的研究开始于20世纪60年代,秀丽线虫作为模式生物是第一个完成基因测序的多细胞生物,普遍应用于各种环境对生理和行为学研究中。空间环境以微重力、强辐射作为特点,对秀丽线虫的生理及行为产生很大影响。本文总结了微重力和辐射引起秀丽线虫运动能力、寿命、能量代谢等方面基因表达变化的研究成果。秀丽线虫与人类的序列相似性高达40%,空间环境对秀丽线虫行为及生长发育的研究为空间环境对人类健康影响研究提供数据支持,也为空间损伤修复研究提供理论基础。     

太空环境下哺乳动物胚胎发育和生殖研究进展及展望

随着人类太空探索进程的加速和深入,哺乳动物能否在太空完成生命孕育和后代繁衍成为科学界及公众关注的问题.过往研究提示,太空飞行会对哺乳动物胚胎发育和生殖功能造成某些潜在的危害,这些危害的产生与太空存在的特殊环境有关,如宇宙辐射和重力等变化.本文首先综述了国内外利用空间飞行器搭载平台、地基微重力和辐射平台开展哺乳动物生殖和发育研究的进展,还特别论述了本团队利用实践十号(SJ-10)返回式科学卫星开展的太空条件下哺乳动物早期胚胎体外发育研究结果,随后展望了未来借助科学实验卫星、空间站、月球和火星探测等太空飞行实验平台进行动物生殖功能和胚胎发育研究的着重点.未来要实现哺乳动物乃至人类在地外空间的生存繁衍,阐明微重力、宇宙辐射或其他空间环境因素对哺乳动物胚胎发育和生殖生理的影响是至关重要的,在此基础上方可采取各种有针对性的保护措施,成功实现地外生命繁衍.     

乙酰胆碱门控氯离子通道受体突变影响秀丽线虫运动学和运动状态转换

目的 乙酰胆碱作为一种高度保守的神经递质，在动物的运动行为调控中起着至关重要的作用。乙酰胆碱信号转导异常可导致多种运动功能障碍。然而，乙酰胆碱在运动行为中的抑制性调控机制尚未完全清楚。本文以秀丽隐杆线虫为研究对象，探究乙酰胆碱门控氯离子通道受体亚基（ACC-1、ACC-2、ACC-3、ACC-4）在运动行为中的调控作用。方法 通过将运动追踪、分子遗传学和光遗传学技术相结合，对乙酰胆碱门控氯离子通道受体亚基突变线虫的运动进行分析。结果 研究发现，这些亚基突变会影响线虫前进、后退和转向运动的运动学特征，并且前进过程中线虫身体弯曲幅度也发生了变化。在这些突变线虫的后退过程中光激活RIB中间神经元会导致后退运动延迟终止。结论 这些结果提示，乙酰胆碱门控氯离子通道亚基的调控作用对于维持和调节秀丽隐杆线虫运动状态是必需的。同时，这些亚基可能参与介导RIB中间神经元在秀丽隐杆线虫后退运动中的抑制性调控。本研究为理解乙酰胆碱门控抑制性受体在运动行为中的调控机制提供了新的思路。     

平滑肌肌球蛋白磷酸化与肌动球蛋白功能调节

在有Ｃａ２＋和钙调蛋白存在时,肌球蛋白轻链激酶催化肌球蛋白磷酸化,促使肌动蛋白激活的肌球蛋白（肌动球蛋白）Ｍｇ２＋－ＡＴＰ酶活性显著增加．然而,肌球蛋白磷酸化水平与Ｍｇ２＋－ＡＴＰ酶之间的关系是非线性的,原肌球蛋白可以进一步增加Ｍｇ２＋－ＡＴＰ酶的活性,但仍不改变它们之间的非线性关系．肌球蛋白轻链激酶的合成肽抑制剂抑制了肌球蛋白磷酸化和Ｍｇ２＋－ＡＴＰ酶活性,并导致平滑肌去膜肌纤维的等长收缩张力与速度的降低．结果提示肌球蛋白轻链激酶参与脊椎动物平滑肌收缩的调节过程,肌球蛋白轻链磷酸化作用会引起平滑肌收缩     

微小RNA-499的表达特征及生物学作用

微小RNA-499（mieroRNA-499,miR-499）是近年来发现的肌球蛋白基因编码的miRNA（miRNA encoded by myosingene,myo—miR）家族新成员,目前发现它主要在人和动物的心肌和骨骼肌中表达,同时在其它多种组织中也可以被检测到。miR-499在心肌细胞的分化中起着至关重要的调控作用。在成人心肌和骨骼肌中,miR-499通过促进β-肌球蛋白重链（β—myosin heavy chain,p-MHC）的表达,使肌细胞的氧代谢和耐受力增强。miR-499可能通过不同的信号转导通路,参与了不同的心肌病理过程。此外,miR-499的血清／血浆水平在多种疾病患者中有显著变化,miR-499前体（pre—miR-499）的多态性也与人体对多种疾病的易感性相关,这些使其有望成为某些疾病临床检验的生物学标志物之一。     

双肾双夹肾性高血压大鼠左心室肌球蛋白重链同型异构 …

目的和方法：测定双肾双夹（２Ｋ２Ｃ）肾性高血压大鼠早期,左心室α－肌球蛋白重链（α－ＭＨＣ）和β－肌球蛋白重链（β－ＭＨＣ）ｍＲＮＡ水平的变化。实验分四组：对照组、２Ｋ２Ｃ组、巯甲丙脯酸组、巯甲丙脯酸对照组。术后２４ｈ、３６ｈ、４８ｈ、７２ｈ测动脉血压,提取左心室中样本取８．０μｇ,与＾３２Ｐ标记的α－ＭＨＣ和β－ＭＨＣ ｃＤＮＡ探针作班点杂交。结果：高血压大鼠左心室α－ＭＨＣ ｍＲＡ水平明显降低     

基于模式生物秀丽隐杆线虫的三丁基锡生态毒性评价

本研究利用秀丽隐杆线虫半致死浓度分析和致死曲线分析来筛选对三丁基锡（Tributyltin,TBT）敏感的线虫品系,并讨论与TBT毒理学过程可能相关的基因。通过对秀丽隐杆线虫体长、每窝子代数和怀卵量的测定来探讨TBT的生态毒性效应,以期为TBT对秀丽隐杆线虫和人类的生态毒性评价和致毒机理研究提供科学依据。结果表明：TBT对各品系线虫48 h LC50从小到大依次为egl-1（n487）＜ced-4（n1162）＜cep-1（gk138）=cep-1（lg12501）＜ced-9（n1950）＜clk-2（mn159）＜ced-3（n717）＜N2＜opIs34（hus-1::GFP） ＜opIs56（egl-1::GFP）＜daf-16（mn86）＜hus-1（op241）＜daf-2（e1370）。本研究筛选出对TBT最敏感的线虫品系为egl-1（n487）,而对TBT耐受力最强的是daf-2（e1370）。TBT对秀丽隐杆线虫体长、每窝子代数和怀卵量均呈现浓度依赖型的抑制作用。     

维生素C通过胰岛素信号通路增强秀丽隐杆线虫抗氧化作用

目的：利用秀丽隐杆线虫为模式生物,研究维生素C在秀丽隐杆线虫体内的抗氧化效应及其机制。方法：分别以含有0.05、0.25、0.5 mg/mL维生素C的NGM培养基饲养秀丽隐杆线虫,测定不同浓度维生素C饲养线虫体内超氧化物歧化酶（SOD）和过氧化氢酶（CAT）的含量,同时检测0.25 mg/mL的维生素C饲养线虫age-1、daf-2、daf-16、sir-2.1、clt-1基因mRNA变化。在高氧环境中,干扰0.25 mg/mL维生素C饲养线虫daf-2、daf-16基因表达检测线虫的存活情况,观察0.25 mg/mL维生素C饲养线虫DAF-16入核情况。结果：0.25 mg/mL的维生素C提高秀丽隐杆线虫体内SOD和CAT活力,在高氧环境中,0.25 mg/mL的维生素C降低age-1、daf-2基因表达,提高daf-16基因表达,同时增加DAF-16蛋白入核。结论：维生素C通过DAF-16胰岛素信号通路增强秀丽隐杆线虫抗氧化作用。     

鸭肫平滑肌肌球蛋白经α－糜蛋白酶轻微酶解及其Mg~（2＋）－ATP酶性质的改变

用α－糜蛋白酶对鸭肫平滑肌肌球蛋白进行有限酶解,使肌球蛋白重链的电泳双带变成单带。酶解后肌球蛋白与正常肌球蛋白相比,肌动蛋白激活的磷酸化肌球蛋白的Ｍｇ２＋－ＡＴＰ酶活力在低Ｍｇ２＋离子浓度时反而较高。从酶解后肌球蛋白溶液中只分离到１个４．２ｋｄ的小肽段。氨基酸组成测定及荧光胺末端标记实验提示,该小肽段酶切自平滑肌肌球蛋白重链ＳＭ１的Ｃ末端。     

Genetic suppression of phenotypes arising from mutations in dystrophin-related genes in Caenorhabditis elegans

BACKGROUND: Dystrophin is the product of the gene that is mutated in Duchenne muscular dystrophy (DMD), a progressive neuromuscular disease for which no treatment is available. Mice carrying a mutation in the gene for dystrophin (mdx mice) display only a mild phenotype, but it is aggravated when combined with a mutation in the MyoD gene. The nematode worm Caenorhabditis elegans has a dystrophin homologue (dys-1), but null mutations in dys-1 do not result in muscle degeneration.RESULTS: We generated worms carrying both the dys-1 null mutation cx18, and a weak mutation, cc561ts, of the C. elegans MyoD homologue hlh-1. The double mutants displayed a time-dependent impairment of locomotion and egg laying, a phenotype not seen in the single mutants, and extensive muscle degeneration. This result allowed us to look for genes that, when misexpressed, could suppress the dys-1; hlh-1 phenotype. When overexpressed, the dyc-1 gene - whose loss-of-function phenotype resembles that of dys-1 - partially suppressed the dys-1; hlh-1 phenotype. The dyc-1 gene encodes a novel protein sharing similarities with the mammalian neural nitric oxide synthase (nNOS)-binding protein CAPON, and is expressed in the muscles of the worm. CONCLUSIONS: As a C. elegans model for dystrophin-dependent myopathy, the dys-1; hlh-1 worms should permit the identification of genes, and ultimately drugs, that would reverse the muscle degeneration in this model.     

A Screen for Genetic Loci Required for Body-Wall Muscle Development during Embryogenesis in Caenorhabditis Elegans

We have used available chromosomal deficiencies to screen for genetic loci whose zygotic expression is required for formation of body-wall muscle cells during embryogenesis in Caenorhabditis elegans. To test for muscle cell differentiation we have assayed for both contractile function and the expression of muscle-specific structural proteins. Monoclonal antibodies directed against two myosin heavy chain isoforms, the products of the unc-54 and myo-3 genes, were used to detect body-wall muscle differentiation. We have screened 77 deficiencies, covering approximately 72% of the genome. Deficiency homozygotes in most cases stain with antibodies to the body-wall muscle myosins and in many cases muscle contractile function is observed. We have identified two regions showing distinct defects in myosin heavy chain gene expression. Embryos homozygous for deficiencies removing the left tip of chromosome V fail to accumulate the myo-3 and unc-54 products, but express antigens characteristic of hypodermal, pharyngeal and neural development. Embryos lacking a large region on chromosome III accumulate the unc-54 product but not the myo-3 product. We conclude that there exist only a small number of loci whose zygotic expression is uniquely required for adoption of a muscle cell fate.     

Comparison of soleus muscles from rats exposed to microgravity for 10 versus 14 days

 The effects of two different duration spaceflights on the extent of atrophy, fiber type composition, and myosin heavy chain (MHC) content of rat soleus muscles were compared. Adult male Fisher rats (n=12) were aboard flight STS-57 and exposed to 10 days of microgravity and adult ovariectomized female Spraque-Dawley rats (n=12) were aboard flight STS-62 for 14 days. Soleus muscles were bilaterally removed from the flight and control animals and frozen for subsequent analyses. Muscle wet weights, fiber types (I, IC, IIC, and IIA), cross-sectional area, and MHC content were determined. Although a significant difference was found between the soleus wet weights of the two ground-based control groups, they were similar with regard to MHC content (ca 90% MHCI and ca 10% MHCIIa) and fiber type composition. Unloading of the muscles caused slow-to-fast transformations which included a decrease in the percentage of type I fibers and MHCI, an increase in fibers classified as type IC, and the expression of two fast myosin heavy chains not found in the control rat soleus muscles (MHCIId and MHCIIb). Although the amount of atrophy (ca 26%) and the extent of slow-to-fast transformation (decrease in the percentage of MHCI from 90% to 82.5%) in the soleus muscles were similar between the two spaceflights, the percentages of the fast MHCs differed. After 14 days of spaceflight, the percentage of MHCIIa was significantly lower and the percentages of MHCIId and MHCIIb were significantly higher than the corresponding MHC content of the soleus muscles from the 10-day animals. Indeed, MHCIId became the predominant fast MHC after 14 days in space. These data suggest fast-to-faster transformations continued during the longer spaceflight. Accepted: 8 January 1998     

Functional and cellular adaptation to weightlessness in primates

Considerable data has been collected on the response of hindlimb muscles to unloading due to both spaceflight and hindlimb suspension. One generalized response to a reduction in load is muscle fiber atrophy, although not all muscles respond the same. For example, predominantly slow extensor muscles like the Sol exhibit a large reduction in fiber size to unloading, while fast extensors like the plantaris and fast flexors like the tibialis anterior show little, if any, atrophy. Our understanding of how muscles respond to microgravity, however, has come primarily from the examination of hindlimb muscles in the unrestrained rat in space. The non-human primate spaceflight paradigm differs considerably from the rodent paradigm in that the monkeys are restrained, usually in a sitting position, while in space. Recently, we examined the effects of microgravity on muscles of the Rhesus monkey by taking biopsies of selected hindlimb muscles prior to and following spaceflights of 14 and 12 day durations (Cosmos 2044 and 2229). Our results revealed that the monkey's response to microgravity differs from that of the rat. The apparent differences in the atrophic response of the hindlimb muscles of the monkey and rat to spaceflight may be attributed to 1) a species difference, 2) a difference in the manner in which the animals were maintained during the flight (i.e., chair restraint or "free-floating"), and/or 3) an ability of the monkeys to counteract the effects of spaceflight with resistive exercise.     

Knockdown and overexpression of Unc-45b result in defective myofibril organization in skeletal muscles of zebrafish embryos

Background  

Unc-45 is a myosin chaperone and a Hsp90 co-chaperone that plays a key role in muscle development. Genetic and biochemical studies in C. elegans have demonstrated that Unc-45 facilitates the process of myosin folding and assembly in body wall muscles. Loss or overexpression of Unc-45 in C. elegans results in defective myofibril organization. In the zebrafish Danio rerio, unc-45b, a homolog of C. elegans unc-45, is expressed in both skeletal and cardiac muscles. Earlier studies indicate that mutation or knockdown of unc-45b expression in zebrafish results in a phenotype characterized by a loss of both thick and thin filament organization in skeletal and cardiac muscle. The effects of unc-45b knockdown on other sarcomeric structures and the phenotype of Unc-45b overexpression, however, are poorly understood in vertebrates.     

The effects of 10 days of spaceflight on the shuttle Endeavour on predominantly fast-twitch muscles in the rat

The primary purpose of this investigation was to determine the effects of microgravity on muscle fibers of the predominantly fast-twitch muscles in the rat. Cross sectional area and myosin heavy chain (MHC) composition were assessed in order to establish the acute effects of microgravity associated with spaceflight. The extensor digitorum longus (EDL) and gastrocnemius muscles were removed from 12 male Fisher 344 rats which had undergone 10 days of spaceflight aboard the space shuttle Endeavor and from 12 age- and weight-matched control animals. Both groups of animals received similar amounts of food and water and were synchronized for photoperiods, environmental temperature, and humidity. Significant (P < 0.05) reductions in muscle fiber size were observed in the gastrocnemius (fiber types I, IIA, IIDB, and IIB) and EDL (fiber type IIB) muscles after spaceflight. Significant MHC isoform transformations also resulted during this brief period of microgravity exposure with a significant decrease in MHC IId isoform in the EDL muscle. A significant decrease was also observed in the MHC IId isoform in the superficial (white) component of the gastrocnemius muscle after spaceflight, although no alterations in MHC profile were demonstrated in the deep (red) component of this muscle. These findings highlight the rapid plasticity of skeletal muscle during short-term spaceflight. If such pronounced adaptations to spaceflight also occur in humans, then astronauts are likely to suffer severe decrements in skeletal muscle performance with long-term space flight and upon return to earth after both short- and long-term missions. Thus, countermeasures aimed at slowing or even preventing muscle fiber atrophy are warranted.     

Myosin heavy chain gene amplification as a suppressor mutation in Caenorhabditis elegans

Summary In the nematode, Caenorhabditis elegans, the body wall muscles contain paramyosin and two different types of myosin heavy chain, MHC A and MHC B. In mutants that do not express MHC B or that express defective paramyosin, muscle structure is disrupted and movement is impaired. Second site mutations in the sup-3 locus partially reverse these defects and are correlated with a 2- to 3-fold increase in the accumulation of the MHC A isoform. The sup-3 mutations occur at a high frequency (10^–4) after ethyl methanesulfonate (EMS) mutagenesis. This is comparable to the average EMS-induced mutation rate per gene in C. elegans. In this paper we show that the sup-3 mutation is an amplification of the structural gene for the MHC A protein, myo-3. We employed genomic Southern hybridization with MHC gene-specific probes in order to measure the copy number of the myo-3 gene relative to that of the MHC B gene, unc-54. We have identified the putative amplification junctions for these sup-3 alleles using a set of cosmid clones which encompass myo-3 region. Although it has been suggested that gene amplification plays an important role in evolution, there are few known cases of gene amplification in the germ line cells of multicellular organisms. The results shown here provide a clear example of a heritable gene amplification event that occurs at a high frequency in the germ line. Similar events may thus represent the initial event in the evolution of new function and in the formation of multigene families.     

Synergy between stresses: an interaction between spaceflight‐associated conditions and the microgravity response

Gravity is the one constant, ubiquitous force that has shaped life on Earth over its 4.8 billion years of evolution. But the sheer inescapability of Earth’s gravitational pull has meant that its influence on Earth’s organisms is difficult to study. Neutralization of the gravity vector (so‐called simulated microgravity) by random movement in three‐dimensional space is the best option for Earth‐based experiments, with spaceflight alone offering the possibility to assess the effects of an extremely reduced gravitational field (microgravity). However, the technical constraints associated with spaceflight introduce complications that can compromise the interpretation of microgravity experiments. It can be unclear whether changes detected in these experiments reflect additional spaceflight‐related stresses (temperature shifts, vibrational effects, radiation exposure, and so on) as opposed to the loss of gravitational force per se. In this issue, Herranz et al. (2010) report a careful study in which the effects of simulated and actual microgravity on gene expression in Drosophila melanogaster were compared and the effects of the flight‐associated stresses on the microgravity responses were investigated. A striking finding emerged. The additional stresses associated with the spaceflight experiment altered the response to microgravity. Despite controlling for the effects of these stresses/constraints, the group found that responses to microgravity are much stronger in the stressed/constrained background than in its absence. This interaction of gravity with other environmental influences is a novel finding with important implications for microgravity research and other situations where multiple stress factors are combined.