萱草花粉中微管蛋白生物化学性质

微管（microtubule）是细胞骨架的重要成份,参与囊泡运输、信息传递等多种生命活动。我们从萱草花粉中纯化了植物微管蛋白,对其生物化学及生物物理学部分性质研究表明,纯化的微管蛋白经超离心法测定沉降系数为6．2S,SDS-PAGE分析α,β微管蛋白分子量为56kD、58kD,凝胶扫描分析纯度为93．7％。等电聚焦电泳测定等电点为pI=5．35。光谱学性质研究结果表明,最大紫外吸收峰为280．8nm,荧光光谱研究表明最大激发波长为282nm;此时的最大发射峰为338nm,圆二色光谱分析二级结构表明小螺旋占27．24％,β-折叠占24．48％,无规卷曲为48．28％,呈典型球蛋白特征。     

结核分枝杆菌重组38kD蛋白用于新疆南疆维吾尔族和湖南湘中汉族血清学诊断的研究

目的：对结核分枝杆菌38kD蛋白编码基因进行克隆表达及纯化,建立基于重组38kD蛋白的酶联免疫吸附法（EusA）检测结核病人血清标本,评价重组38kD蛋白用于结核病血清学诊断抗原的价值。并比较分析其在汉族和维吾尔族人群中的血清学诊断的差异。方法：用PCR方法扩增38kD蛋白的编码基因,构建重组质粒,转化到大肠杆菌BL21中,经IPTG诱导表达,得到纯化的38kD蛋白,建立以38kD蛋白为包被抗原的ELISA,并检测临床确诊的结核病人血清标本。结果：ELISA检测结核病患者血清标本的维吾尔族阳性率为34％（52／153）,汉族为52．4％（65／124）,两者对比有统计学差异（x2=9．538,P〈O．005）。在阴性对照中的维吾尔族特异度为96．4％（159／165）,汉族为98．8％（130／133）,结果无统计学意义（x2=0．111,P〉0．5）。结论：重组38kD蛋白用于血清学诊断的敏感度在维吾尔族和汉族中有差异,而其诊断特异度无差别。     

绿豆芽中微管蛋白异型的研究

采用 DEAE-Sephadex-A50离子交换层析和 PGGE 电泳对绿豆(Phaseolus radiatus L.)芽中的微管蛋白进行分离。Western blot 和免疫点印迹分析发现了两种聚合度不同的微管蛋白异型。单体微管蛋白亚基的分子量为56kD 和56.5kD;四聚体微管蛋白亚基的分子量为54kD 和54.5kD。实验结果表明微管蛋白α、β亚基组装过程是一个相互选择的过程,这种现象可能与微管蛋白基因表达有关。     

萱草花粉动力蛋白的分离与特性

动力蛋白（dynamin）是一类具有可被微管激活的GTP酶活性的新型马达蛋白,被证明在动物细胞受体介导的内吞小泡的形成,突触小泡再循环及高尔基体的囊泡运输中起关键作用。近几年,一些植物细胞也被发现有动力蛋白类似物。本研究通过分子量鉴定和免疫印迹法证明萱草（Hemerocallis fulva L.)花粉中存在动力蛋白,其分子量为100kD。经过高度纯化的花粉动甩具有GTPase活性,且可被牛脑微管激活1．64倍;电子显微镜表明,花粉动力蛋白可自我组装成环状结构。     

肾综合征出血热纯化疫苗的SDS-PAGE分析

为了证明蛑综合征出血热纯化疫苗的主要成分坦病毒蛋白,采用出血热纯化疫苗经浓缩后进行SDS－PAGE和Western-blotting分析。结果 经SDS－PAGE显示,肾综合征出血热纯化疫苗有三条蛋白带,分子量分别约为70kD、55kD和50kD,与汉坦病毒三种结构蛋白（糖蛋白G1、G2和核蛋白NP）的分子量相符;经Western-blotting显示,分子量50kD的蛋白带反应阳性,分子量70kD和55kD的蛋白带无反应,认定出血热纯化疫苗的主要成分为汉坦病毒蛋白,主要由G1、G2和NP三种结构蛋白构成。     

棉铃虫中肠微粒体P450的分离纯化

为深入研究棉铃虫Helicoverpa armigera细胞色素P450的结构与功能,需要分离不同型的P450蛋白。作者建立了适用于棉铃虫中肠微粒体P450的纯化方法,包括聚乙二醇8000（PEG8000）沉淀、高效疏水作用色谱（HPHIC）和高效离子交换色谱（HPIEC）等连续分离步。SDS-PAGE（银染）显示,棉铃虫中肠微粒体经以上步骤分离纯化后,在含P450的馏分中检测出分子量分别为58 kD、47 kD、56 kD和45 kD的4条蛋白带。 P450的回收率为14.3%,比含量提高了39倍。     

霜霉菌或水分胁迫诱导的黄瓜叶片胞间隙27kD蛋白为几丁质酶

蛋白含量测定和十二烷基硫酸钠．聚丙烯酰胺凝胶电泳（SDS-PAGE）分析结果表明,水分胁迫或霜霉菌接种处理均使黄瓜（Cucumis sativus L.）叶片胞间隙总蛋白含量升高,27kD蛋白积累。通过基体辅助激光解析电离飞行时间质谱0VIALDI-TOFMS）分析纯化的27kD蛋白,将所得的PMF（肽指纹图谱）在NCBInr蛋白质数据库中比对,发现水分胁迫和霜霉菌接种所诱导的27kD蛋白是同一种蛋白,均为一种酸性的几丁质酶。其酶活性测定结果表明,水分胁迫或霜霉菌接种处理的叶片胞间隙液几丁质酶活性均高于对照。     

2（4′噻唑）苯丙咪唑对猪脑微管蛋白体外聚合的影响

本研究利用猪脑中分离纯化的微管蛋白聚合和解聚反应,分析了具有争议的非整倍体诱发剂2（4′噻唑）苯丙咪唑（thiabendazole,TBZ）对微管蛋白聚合状态的影响。秋水仙素(colchicine)为本研究的阳性对照物。结果发现2（4′噻唑）苯丙咪唑能显著抑制体外微管蛋白的聚合,并呈明显的剂量效应关系。研究表明,TBZ可能通过抑制微管蛋白聚合来影响染色体正常分离,诱发非整倍体。     

人微管结合蛋白4微管结合区的体外表达

目的：构建表达人微管结合蛋白4微管结合区（Microtubule-binding domain,MTB）的大肠杆菌工程菌。方法：将1.27Kb编码MTB的DNA片段按正确方向亚克隆到原核生物表达载体pET-3α。得到表达质粒JS3,并转化大肠杆菌BL21（DE3）。结果：IPTG诱导下,表达产物的SDS-PAGE分子量大约是40kD,并能被抗MAP4抗体特异地识别。此外,重组MTB蛋白能在体外结合微管。结论：人微管结合蛋白4微管结合区具有微管结合活性。     

人肝癌细胞的IGF-BP1分子特性及内源性蛋白酶对其降解的研究

用SDS-PAGE电泳、高效液相色谱（HPLC）、质谱等方法,研究了人肝癌细胞（HepG2）分泌的胰岛素样生长因子结合蛋白-1（35S-IGF-BP1）的分子结构、特性,及其被内源性蛋白酶降解的特点．35S-IGF-BP1经抗体免疫沉淀、生化分离,纯化为均一体．其分子是由多个亚基构成的蛋白质,分子量约为27kD;细胞UMR、HepG2、H35。BRL3A分泌的蛋白酶能将35S-IGF-BP1催化水解成较小分子（14kD）的多肽．     

Interaction of tubulin with octyl glucoside and deoxycholate. 1. Binding and hydrodynamic studies

Tubulin purified from calf brain cytoplasm, normally a compact water-soluble dimer, is able to interact with the mild detergents octyl glucoside (a minimum of 60 detergent molecules) and deoxycholate (95 +/- 8 molecules). Binding is cooperative and approaches saturation below the critical micelle concentration of the amphiphiles. Binding is accompanied by a quenching of the intrinsic protein fluorescence, but no spectral shape changes indicating denaturation such as in the case of sodium dodecyl sulfate are observed. Glycerol, which is known to be preferentially excluded from the tubulin domain and to favor the folded and associated forms of this protein, inhibits the binding of the mild detergents. Octyl glucoside induces a rapidly equilibrating tubulin self-association reaction characterized by a bimodal sedimentation velocity profile with boundaries at approximately 5 and 12 S. Full dissociation of this detergent restores the normal sedimentation behavior to 90% of the protein. Binding of deoxycholate slows the sedimentation velocity of tubulin from s(0)20,w = 5.6 +/- 0.2 S to s(0)20,w = 4.8 +/- 0.3 S. Measurements of the molecular weight of the tubulin-deoxycholate complex indicate an increase from 100,000 to 143,000 +/- 5,000. The diffusion rate consistently decreases from (5.3 +/- 0.5) X 10(-7) to (3.8 +/- 0.2) X 10(-7) cm2 S-1. This is most simply interpreted as an expansion of the undissociated tubulin dimer upon detergent binding (a change in the frictional ratio, f/f min, from 1.35 to 1.86). It is concluded that tubulin shows a reversible transition between the water-soluble state and amphipathic detergent-bound forms which constitute a model system of tubulin-membrane interactions.     

Tubulin and microtubule are potential targets for brain hexokinase binding.

The metabolite-modulated association of a fraction of hexokinase to mitochondria in brain is well documented, however, the involvement of other non-mitochondrial components in the binding of the hexokinase is controversial. Now we present evidence that the hexokinase binds both tubulin and microtubules in brain in vitro systems. The interaction of tubulin with purified bovine brain hexokinase was characterized by displacement enzyme-linked immunosorbent assay using specific anti-brain hexokinase serum (IC(50)=4.0+/-1.4 microM). This value virtually was not affected by specific ligands such as ATP or glucose 6-phosphate. Microtubule-bound hexokinase obtained in reconstituted systems using microtubule and purified hexokinase or brain extract was visualized by transmission and immunoelectron microscopy on the surface of tubules. The association of purified bovine brain hexokinase with either tubulin or microtubules caused about 30% increase in the activity of the enzyme. This activation was also observed in brain, but not in muscle cell-free extract. The possible physiological relevance of the multiple heteroassociation of brain hexokinase is discussed.     

Preparation and characterization of des-C-terminal tubulin

Tubulin, from which the C-terminal peptide had been removed by limited proteolysis was compared to intact native tubulin. Des-C-terminal tubulin (with a nominal molecular weight of 48,000) was prepared by digestion with 1% subtilisin carlsberg at 25°C for 16 min, and the product was purified by ion-exchange chromatography on cellulose DE-52 followed by Sephadex G-50 chromatography. The purified product was composed of the cores of both the - and -subunits of tubulin and was free from other proteins and peptides containing the COOH-terminal moiety as shown by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) Sephadex G-50 and ion exchange DE-52 cellulose chromatographies, and ultracentrifugation analysis. The ultraviolet (UV) absorption and fluorescence spectra of des-C-terminal tubulin were the same as those of native tubulin. The sedimentation coefficient of des-C-terminal tubulin (5.9S) was slightly higher than that of native tubulin reflecting a decrease in axial ratio. The change in circular dichroism in the far UV indicated a decrease of -helical contents by 10–15%. These optical properties of des-C-terminal tubulin indicate that the elimination of the COOH-terminal region from tubulin did not change the conformation of the core tubulin molecule significantly, the decrease in -helix being due to the elimination of the C-terminal peptide. des-C-terminal tubulin bound 2 moles/mole of GTP and 1 mole/mole of colchicine, just as intact tubulin, but its binding ability of ruthenium red was reduced.     

Purification of tau,a microtubule-associated protein that induces assembly of microtubules from purified tubulin

Tau, a microtubule-associated protein which copurifies with tubulin through successive cycles of polymerization and depolymerization, has been isolated from tubulin by phosphocellulose chromatography and purified to near homogeneity. The purified protein is seen to migrate during electrophoresis on acrylamide gels as four closely spaced bands of apparent molecular weights between 55,000 and 62,000. Specific activity for induction of microtubule formation from purified tubulin has been assayed by quantitative electron microscopy and is seen to be enhanced three- to fourfold in the purified tau when compared with the unfractionated microtubule-associated proteins. Nearly 90% of available tubulin at 1 mg/ml is found to be polymerizable into microtubules with elevated levels of tau. Moreover, the critical concentration for polymerization of the reconstituted tau + tubulin system is seen to be a function of tau concentration and may be lowered to as little as 30 μg of tubulin per ml. Under depolymerizing conditions, 50% of the tubulin at only 1 mg/ml may be driven into ring structures. A separate purification procedure for isolation of tau directly from cell extracts has been developed and data from this purification suggest that tau is present in the extract in roughly the same proportion to tubulin as is found in microtubules purified by cycles of assembly and disassembly. Tau is sufficient for both nucleation and elongation of microtubules from purified tubulin and hence the reconstituted tau + tubulin system defines a complete microtubule assembly system under standard buffer conditions. In an accompanying paper (Cleveland et al., 1977) the physical and chemical properties of tau are discussed and a model by which tau may function in microtubule assembly is presented.     

肌动蛋白在丝瓜花粉管顶端生长中的作用

用非固定荧光标记的鬼笔环肽作为肌动蛋白探针观察并证明了丝瓜未萌发的花粉粒和不同生长时期花粉管中肌动蛋白纤丝的分布及其形态变化。又用细胞松弛素B（CB）、氯两嗪（CPZ）及N-乙酰马来酰胺（NEM）证明了丝瓜花粉管伸长与肌动蛋白既有密切的关系,也受Ca2 的调节。     

新疆罂粟属高山罂粟组分类研究

我国有罂粟属植物12种,新疆有10种,其中6种属于高山罂粟组。对新疆高山罂粟组植物的花葶进行了解剖研究,并用扫描电镜观察了花粉形态,结果表明,花葶中维管束的数量及排列方式在各种间存在着差异,可以作为一个鉴定特征。花粉上的小刺密度在放大12000倍时,在有种间存在着明显差异,可分类提供微观佐证。     

A mutant beta-tubulin confers resistance to the action of benzimidazole-carbamate microtubule inhibitors both in vivo and in vitro

The mutant BEN210 of Physarum polycephalum is highly resistant to a number of benzimidazole carbamate agents, including methylbenzimidazole-2-yl-carbamate and parbendazole. The resistance is conferred by the benD210 mutation in a structural gene for beta-tubulin. This mutant allele encodes a beta-tubulin with novel electrophoretic mobility. We have used this strain to determine whether the mutant beta-tubulin is used in microtubules and whether this usage permits microtubule polymerisation in the presence of drugs both in vivo and in vitro. In vitro assembly studies of tubulin purified from the mutant strain have shown that microtubules are formed both in the absence of drugs and in all drug concentrations tested (up to 50 microM parbendazole). In contrast, the assembly of microtubules from wild-type tubulin in vitro is totally inhibited by 2-5 microM parbendazole. Thus the resistance of BEN210 to parbendazole observed in vivo has been reproduced in vitro using tubulin purified from the mutant strain. Electrophoretic analysis of the microtubules formed in vitro has shown that both the wild-type and the mutant beta-tubulin are incorporated into the microtubules and that the proportion of mutant to wild-type beta-tubulin appears to remain constant with increasing drug concentration. This is the first demonstration of a single mutation in a tubulin structural gene causing an altered function of the gene product in vitro.     

Overexpression,purification, and functional analysis of recombinant human tubulin dimer

Microtubules consisting of tubulin dimers play essential roles in various cellular functions. Investigating the structure–function relationship of tubulin dimers requires a method to prepare sufficient quantities of recombinant tubulin. To this end, we simultaneously expressed human α1- and β3-tubulin using a baculovirus-insect cell expression system that enabled the purification of 5 mg recombinant tubulin per litre of cell culture. The purified recombinant human tubulin could be polymerized into microtubules that glide on a kinesin-coated glass surface. The method provides a powerful tool for in vitro functional analyses of microtubules.     

Tubulin-chromatin interactions: evidence for tubulin-binding sites on chromatin and isolated oligonucleosomes

The interaction of tubulin with chromatin has been studied using a radiolabeled tubulin binding assay and velocity sedimentation analysis on isokinetic sucrose gradients. Soluble chromatin was prepared by mild micrococcal nuclease digestion of rat liver nuclei and tubulin was purified from rat brain by temperature-dependent assembly-disassembly and phosphocellulose chromatography. The tubulin-binding assay is based on the ability of chromatin to precipitate quantitatively at physiological ionic strength allowing separation of free tubulin from chromatin-bound tubulin. The binding of tubulin to unfractionated soluble chromatin was rapid, reversible and saturable. Saturation of binding sites was obtained using tubulin concentrations ranging from 0.5 to 400 micrograms/ml, in the presence of a high concentration (2.5 mg/ml) of another acidic protein, bovine serum albumin. The Scatchard and Hill plots showed that tubulin bound to a single class of non-interacting sites and yielded values of (0.5-0.6) X 10(7) M-1 for an apparent Ka and a maximal binding capacity of 0.8 nmol tubulin/mg DNA, i.e. about 1 molecule of tubulin/10 nucleosomes. Similar binding parameters were obtained when binding experiments were performed with insoluble chromatin in 0.15 M NaCl. Velocity sedimentation analysis of tubulin-chromatin complexes revealed that tubulin bound to all classes of chromatin oligomers, irrespective of the length of the nucleosomal chain. Tubulin-trinucleosome complexes formed from isolated trinucleosome in the presence of an excess of tubulin were separated from free reactants. It was found that 10-15% of the starting oligonucleosomal species reacted with tubulin, in a stoichiometry of about 0.8 molecule of tubulin/nucleosome. Given the characteristics of the binding and the expected cellular free tubulin concentration, the tubulin-chromatin interaction could possibly take place in vivo, when the nuclear membrane breaks down during the first steps of mitosis.     

Chemical modification of bovine brain tubulin with the guanine nucleotide affinity analogue 5'-p-fluorosulfonylbenzoylguanosine

Bovine brain tubulin purified in the absence of GTP and MgCl2, reacts with 5'-p-fluorosulfonylbenzoylguanosine (5'-FSBG)2, an affinity analog of GTP and two moles of the reagent are incorporated per mole of tubulin at 0 degree C. 5'-FSBG is unable to promote the polymerization of tubulin into microtubules. 2 mM GTP, podophyllotoxin and vinblastine provide almost 50% protection against the modification, when added individually. Combination of these ligands gives maximal protection. Tubulin modified with 5'-FSBG lost two sulfhydryl groups per mole of tubulin and reduction with beta-mercaptoethanol led to the loss of the 2 moles of FSBG that had been incorporated. These data are interpreted on the basis that the modification of tubulin by 5'-FSBG proceeds via a thiosulfonate intermediate between the analogue and a reactive thiol group at or near that portion of the GTP binding site of tubulin where the phosphate moiety of GTP binds.