一种改良的肌细胞骨架染色方法

为了观察肌细胞骨架,对传统考马斯亮蓝染色法进行改良,并与免疫荧光染色法进行了比较。培养的血管平滑肌细胞先用多聚甲醛预固定后再进行考马斯亮蓝染色,可使细胞骨架非常清晰的显色,解决了传统考马斯亮蓝染色易使肌细胞变形、脱片的问题,其效果与免疫荧光染色相近。因此,多聚甲醛预固定．考马斯亮蓝染色法是一种适于肌细胞骨架染色的简便方法。     

绿豆根尖细胞微管骨架有丝分裂时相发育变化的研究

提纯猪脑微管蛋白,制备兔抗微管蛋白抗血清,以此抗体与羊抗兔ｌｇＧ－ＦＩＴＣ因清,对绿豆根尖细胞进行间接免疫荧光标记和荧光显微镜检,得到了绿豆根尖细胞有丝分裂微管骨架周期发育变化的时相,如：早前期带,纺棰体微管,成膜体微管等,结果证明了双子叶植物具有与单子叶植物相似的细胞分裂微管周期时相,表明了微管架周期时相变化在高等植物中具有普遍性和共同变化的规律,讨论了微管骨架时相发育变化与染色有丝分裂行为的关     

双子叶植物细胞周期微管骨架的时相变化的免疫荧光显微研究

本工作用两个循环的组装－去组装超速离心法提取和纯化猪脑微管蛋白,制备兔抗微管蛋白血清,并首次用免疫荧光显微术,对双子叶植物绿豆根尖细胞周期微管骨架各时相的排布进行了检测和分析。讨论了微管周期和染色体周期的细胞有丝分裂行为。     

用于本科教学的间接免疫荧光法观察玉簪保卫细胞微管骨架

细胞骨架的观察是生命科学类专业本科生一个很重要的实验。目前,在细胞生物学实验教学中常用考马斯亮蓝染色法观察植物细胞骨架,但存在诸多不足。该研究选取洋葱、大叶黄杨、玉簪三种植物材料,利用间接免疫荧光法对微管进行观察比较。结果表明,三种植物中,玉簪作为一种常见的绿化观赏花卉植物,取材方便、撕片容易,其气孔保卫细胞微管骨架免疫荧光图像显示清晰,在低温处理后也可观察到微管解聚现象。因此,玉簪可作为本科生实验教学中利用免疫荧光法观察微管骨架的一种易得、观察效果好的实验材料。     

洋葱鳞茎内表皮细胞中的微管

用超薄切片和原生质体负染的方法,在电镜下观察到洋葱鳞茎内表皮细胞周质微管的存在。其出现时间、分布状况以及排列形态,基本上与考马斯亮蓝染色法观察到的网状结构物相一致。讨论了包被囊泡和微管组织中心可能的作用。     

一种改进的观察植物细胞微管的免疫荧光染色方法

植物微管体积小,而且始终处于动态变化之中,因此观察到清晰的微管形态有一定的难度。本文以拟南芥为实验材料,介绍了一种改进的植物细胞微管免疫荧光染色方法,用此方法可以观察到清晰、完整的植物微管形态,此法对其他植物细胞微管观察可能也有借鉴和参考价值。     

粗茎鳞毛蕨原叶体细胞有丝分裂过程中微管列阵的变化

应用Steedman‘s wax切片法,间接免疫荧光标记技术和激光共聚焦扫描显微镜技术研究了粗茎鳞毛蕨（Dryopteris crassirhizoma Nakai)原叶体大液泡化细胞和分生组织细胞有丝分裂过程中微管列阵的变化。结果显示：应用高浓度的多聚甲醛（8%）可以很好地保持大液泡化细胞的结构和微管的抗原性。结果也显示Steedman‘s wax切片法和间接免疫荧光标记技术的优点;（1）避免在微管标记过程中酶解细胞壁;（2）在乙醇脱水过程中样品中叶绿素的自发荧光被减到最小;（3）能够详细观察到有丝分裂过程中微管骨架的变化。因此,这种方法可以被广泛用来调查简单植物体和复杂植物体中细胞的有丝分裂过程以及发育过程中微管骨架的变化。     

离子束注入对细胞有丝分裂微管骨架影响的研究

经能量为２０～３０Ｋｅｖ注入剂量为６×１０１５Ｎ＋／ｃｍ２和１０×１０１５Ｎ＋／ｃｍ２的Ｎ＋离子注入及免疫荧光抗体标记显微观察和统计,结果表明,在绿豆根尖细胞有丝分裂中,分裂细胞的形体、中后期细胞数目、细胞微管骨架以及纺缍体的排布方式均发生了异常变化。１２－１３％的分裂细胞个体增大,８－１０％有丝分裂中后期细胞数目高于对照组,间期细胞微管骨架荧光强度明显弱于对照组,且有２－４％的较强荧光小体和无荧光小体（微孔洞,ｍｉｃｒｏｏｐｅｎｉｎｇ）。３－１２％的中后期细胞中出现不对称和极向不同步移动排布的纺缍体。研究结果表明：２０～３０Ｋｅｖ的能量和剂量为６～１０×１０１５Ｎ＋／ｃｍ２的Ｎ＋离子束注入,对绿豆根尖细胞有丝分裂微管骨架可诱发产生异常变化,同时也可以初步认为这种变化结果与Ｎ＋离子束注入产生的染色体异常分配和运动功能活动有密切的相关性。     

沉默黏着斑激酶促进人胃癌SGC-7901细胞骨架蛋白解聚及细胞形态损伤

目的探讨黏着斑激酶(focal adhesion kinase,FAK)在胃癌细胞骨架结构及形态结构维持中的作用。方法利用靶向FAK的siRNA质粒,转染胃癌SGC-7901细胞,用罗丹明标记的鬼笔环肽及β-tubulin特异性抗体检测细胞骨架微丝及微管蛋白表达;考马斯亮蓝染液对细胞进行染色,观察细胞整体形态结构;环境扫描电子显微镜观察细胞表面结构。结果沉默FAK引起细胞质、细胞伪足及微绒毛等运动相关结构中F-actin解聚。随着沉默时间增长,围绕着细胞核,在细胞质中呈放射状的微管骨架发生解聚,且这种解聚现象呈时间依赖性。FAK沉默还使细胞由梭形、多边形变为圆形,发生脱壁;细胞微绒毛及伪足结构受损,细胞表面趋于光滑。结论 FAK对维持胃癌细胞微丝、微管的分布及癌细胞伪足、微绒毛等恶性形态学特征具有重要作用。     

小麦叶肉细胞原生质体中微管骨架的排列格局与[Ca2+]cyt的关系

以小麦叶肉细胞原生质体为材料,通过免疫荧光标记和Ca~(2 )荧光染料的装载并结合药物学试验,借助激光共聚焦扫描显微镜观察,探讨微管骨架和Ca~(2 )之间的内在联系。试验结果表明,[Ca~(2 )]_(cyt)的升高能够诱发微管骨架的解聚;而微管骨架的解聚也会促使胞外Ca~(2 )内流,进而造成[Ca~(2 )]_(cyt)的升高。     

大鼠SUMO特异性蛋白酶1催化区蛋白制备及功能鉴定*

目的: 制备大鼠SUMO特异性蛋白酶1(sentrin-specific protease,SENP1)催化结构域(SENP1C)蛋白,并鉴定其酶活性。方法: 分别以大鼠SENP1-pcDNA3.1和EGFP-pcDNA3.1重组体为模板,PCR扩增目的基因,克隆入pGEM-T载体;酶切鉴定后,再亚克隆入原核表达载体pET-28a;阳性重组体导入原核表达细胞BL-21,异丙基硫半乳糖苷(IPTG)诱导蛋白质表达;SDS-PAGE及考马斯亮蓝染色鉴定蛋白质的表达。Ni-NTA吸附纯化蛋白质并透析处理,SDS-PAGE及考马斯亮蓝染色鉴定蛋白质的纯度;1 μmol/L及5 μmol/L Tat-EGFP分别孵育HT22细胞不同时间,荧光显微镜下观察细胞转染情况。采用5 μmol/L Tat-SENP1C预孵育HT22细胞10 h,免疫印迹检测整体蛋白质的SUMO化水平;用5 μmol/L Tat-SENP1C预孵育HT22细胞或过表达Myc-Akt1和HA-SUMO1的HT22细胞10 h后,免疫沉淀和免疫印迹检测内源性和外源性Akt1与SUMO1的结合(SUMO化)。结果: Tat-SENP1C-pET-28a和Tat-EGFP-pET-28a重组原核表达载体成功构建,IPTG可以诱导蛋白质高表达;采用Ni-NTA纯化和透析可获得较高纯度的蛋白质;5 μmol/L Tat-EGFP孵育HT22 细胞10 h后,蛋白质穿膜效率较高;Tat-SENP1C重组蛋白可以显著降低HT22细胞中整体蛋白质的SUMO化以及内源性和外源性Akt1 SUMO化。结论: Tat-SENP1C-pET-28a和Tat-EGFP-pET-28a重组原核表达载体构建成功,且被IPTG诱导后可高效表达蛋白质;纯化的Tat-SENP1C蛋白具有较强的穿膜能力及酶活性。     

Influence of the protein staining in the fast ultrasonic sample treatment for protein identification through peptide mass fingerprint and matrix-assisted laser desorption ionization time of flight mass spectrometry

The influence of the protein staining used to visualize protein bands, after in-gel protein separation, for the correct identification of proteins by peptide mass fingerprint (PMF) after application of the ultrasonic in-gel protein protocol was studied. Coomassie brilliant blue and silver nitrate, both visible stains, and the fluorescent dyes Sypro Red and Sypro Orange were evaluated. Results obtained after comparison with the overnight in-gel protocol showed that good results, in terms of protein sequence coverage and number of peptides matched, can be obtained with anyone of the four stains studied. Two minutes of enzymatic digestion time was enough for proteins stained with coomassie blue, while 4 min was necessary when silver or Sypro stainings were employed in order to reach equivalent results to those obtained for the overnigh in-gel protein protocol. For the silver nitrate stain, the concentration of silver present in the staining solution must be 0.09% (w/v) to minimize background in the MALDI mass spectra.     

甘蔗茎尖细胞有丝分裂过程中微管骨架的变化

利用改进的冰冻切片法结合间接免疫荧光标记技术对甘蔗茎尖细胞有丝分裂过程中微管骨架的变化进行了研究。结果表明,在甘蔗茎尖细胞有丝分裂过程中存在4种循序变化的典型微管列阵,即周质微管、早前期微管带、纺锤体微管及成膜体微管。同时,还观察到在各种典型微管列阵相互转变过程中存在各种微管列阵的过渡状态。甘蔗茎尖正在伸长的幼叶部位细胞的周质微管主要为与细胞伸长轴相垂直的横向周质微管：茎尖幼叶部位伸长缓慢细胞的微管主要为纵向及斜向排列的周质微管,在甘蔗茎尖幼叶基部初生增粗分生组织处,横向、斜向、纵向及随机排列的周质微管列阵均有分布。在少数分裂前期的细胞中,发现细胞具有2条早前期微管带,其具体功能还不清楚。表明甘蔗茎尖细胞微管列阵的变化与许多双子叶植物及部分单子叶植物具有共同的变化规律,进一步证明微管骨架的周期性变化在植物中具有普遍性。     

Tyrosinated, but not detyrosinated, α-tubulin is present in root tip cells

Summary The distribution of tyrosinated and detyrosinated tubulin in microtubule arrays of pine and onion cells was investigated by immunofluorescence techniques. Staining of isolated cells and methacrylate sections ofPinus radiata andAllium cepa root tips indicated that all microtubule structures contained tyrosinated tubulin but not the posttranslationally modified detyrosinated tubulin. The detyrosinated tubulin epitope was, however, created in vitro by treating both sections and fixed whole cells with carboxypeptidase A.     

Effect of cold exposure on cortical microtubules of rye (Secale cereale) as observed by immunocytochemistry

The responses of cortical microtubules to sub-zero temperatures were examined in non-acclimated (NA) and cold-acclimated (CA) rye ( Secale cereale L. cv. Voima) leaf and root cells, and in protoplasts isolated enzymatically from leaves. Responses of leaf and root cells to hypertonic solutions equivalent to the dehydration response of freezing (P. L. Steponkus and D. V. Lynch 1989. J. Bioenerg. Biomembr. 21: 21–41) were also examined. At the respective growth temperatures both NA and CA leaf and root cells had typical organization and abundance of cortical microtubules as observed by indirect immunofluorescence (IIF) staining. Unchanged microtubule arrays were still present in CA leaf cells after -4°C treatment, while in leaf cells of NA plants and in the root cells of both NA and CA plants microtubules were shorter and less abundant. After -10°C treatment the cortical microtubules were almost totally depolymerized in both types of root cells and in leaf cells of NA plants, while CA leaf cells still had abundant cortical microtubule arrays. Semiquantitative analyses of cortical microtubules (MTs) of protoplasts confirmed the findings with intact leaf cells. Hypertonic treatment of NA and CA leaf cells gave similar effects as exposure of cells to sub-zero temperatures. However, after the hypertonic treatment, more microtubules remained present in the CA root cells than in the NA root cells, suggesting that also in root cells cold acclimation increases the dehydration stability of MTs. In conclusion, cold acclimation induces both greater frost stability and greater osmotic tolerance in the cortical microtubules of the leaf cells, and greater osmotic tolerance in the microtubules of the root cells in winter rye.     

Formation of intercellular gas space in the diaphragm during the development of aerenchyma in the leaf petiole of Sagittaria trifolia

The development of aerenchyma in the petiole of Sagittaria trifolia L. was studied by means of light-microscopy, scanning electron microscope, transmission electron microscope and immunofluorescence, focusing on the formation of intercellular spaces in diaphragms and its relationship with the organization of cortical microtubule arrays. A complex and organized honeycomb-like schizogenous aerenchyma formed by cylinders and vascular diaphragms was observed in the petiole of S. trifolia at different developmental stages. Cell division was the primary factor contributing to the increased volume of air spaces at early stages, while cell enlargement became the primary factor at later stages. The cortical microtubules localize at the sites where intercellular spaces and the secondary cell walls will be formed or deposited during the formation of intercellular spaces by the separation of diaphragm cells. Cortical microtubules were observed at the boundary of diaphragm cells and the fringes of intercellular spaces at later developmental stages where cell expansion occurs rapidly. These observations support the hypothesis that reorganization of cortical microtubule arrays might be related to the formation of air spaces in diaphragms and are involved in the deposition of secondary cell walls.     

Microtubule Cycle in Root Tip Cells of Allium fistulosum L.

Using immunofluorescent localization techniques and TEM methods, the organization of microtubule arrays during the cell cycle of root tip cells of Allium fistulosum L. was studied. There are four basic types of microtubule organization, namely, interphase cortical microtubule, pre-prophase band microtubule, spindle microtubule and phragmoplast microtubule, which constitute the typical microtubule cycle in dividing cells of higher plants. The fluorescent figures of microtubules observed under fluorescent microscope were explained and analysed by the ultrastractural informations of microtubules obtained from TEM.     

A blue dive: from ‘blue fingers’ to ‘blue silver’. A comparative overview of staining methods for in-gel proteomics

Gel-based proteomics are the most useful method for protein separation, even when compared with gel-free proteomics. Proteomic analysis by 2D gel electrophoresis (2-DE) with immobilized pH gradients is in turn the best approach to large-scale protein-expression screening. Spots visualization is pivotal for protein identification by mass spectrometry. Commonly used staining methods with excellent mass spectrometry compatibility are coomassie brilliant blue (CBB) or fluorescent dyes. In this study, an implementation of ‘blue silver’ colloidal CBB staining, characterized by high sensitivity and immediate low background, is discussed. The sensitivity of classical, colloidal and ‘blue silver’ CBB staining methods was compared on monodimensional and 2-DE gels. The implementation of the ‘blue silver’ method performs better, provided the physical state of the micelles is respected. An example of a 2-DE of human urine treated with combinatorial peptide ligand libraries demonstrates that implemented ‘blue silver’ can evidence the complexity of the sample.