老年大鼠与断奶大鼠脑细胞核染色质的非组蛋白研究

用不连续盘状SDS-聚丙烯酰胺凝胶电泳分析并比较了老年大鼠与断奶大鼠脑细胞核NHCP,也比较了二者的组蛋白与DNA、NHCP与组蛋白、NHCP与DNA之比值。发现老年大鼠NHCP含量明显减少;断奶大鼠的NHCP与DNA、NHCP与组蛋白之比值明显高于老年大鼠,而组蛋白与DNA之比值却近于1。从二者的NHCP电泳图谱可见,老年大鼠丢失了表观分子量10万以上的两条蛋白区带及表观分子量3万以下的一条蛋白区带;老年大鼠与断奶大鼠比较,表观分予量6—9万的蛋白区带杂色浅,而表观分子量4.3万的蛋白区带染色深。总之,老年大鼠脑细胞核NHCP发生质与量的变化。     

MMP-2及TIMP-2的表达与胶质瘤复发相关性的研究

目的:探讨基质金属蛋白酶类与胶质细胞瘤浸润性生长之间的关系及其在胶质瘤复发中的作用。以及基质金属蛋白酶及其抑制因子(MMP-2、TIMP-2)的阳性表达与胶质细胞瘤病理分级及预后的关系。方法:应用免疫组织化学染色法(SP法)检测48例人脑原发和复发胶质细胞瘤组织中MMP-2、TIMP-2的表达。结果:Ⅲ、Ⅳ级和复发胶质细胞瘤中的MMP-2蛋白的表达显著高于Ⅰ、Ⅱ级(P<0.05);Ⅰ、Ⅱ级胶质细胞瘤中的TIMP-2蛋白的表达显著高于复发胶质细胞瘤(P<0.05)而与Ⅲ、Ⅳ级细胞瘤无显著性差异(P>0.05);Ⅲ、Ⅳ级和复发胶质细胞瘤中的MMP-2,TIMP-2蛋白的表达无显著差异(P>0.05);同级别胶质细胞瘤中MMP-2、TIMP-2的表达之间无明显相关性(P>0.05);正常脑组织中无表达。结论:MMP-2、TIMP-2的表达与胶质细胞瘤的恶性程度有关,低级别中,MMP-2与TIMP-2成正相关;MMP-2的高表达,TIMP-2的低表达与胶质细胞瘤的侵袭有关,MMP-2、TIMP-2的表达水平有可能成为判定胶质细胞瘤恶性程度、侵袭能力和预后的诊断指标,而且TIMP-2可能更加敏感。     

黄鳝性逆转与性腺蛋白关系的分析

实验采用聚丙烯酰胺梯度胶电泳方法，对２６２黄鳝的性腺蛋白进行了分析，结果表明雌性黄鳝随着性腺的成熟性腺蛋白组分有所增多，相反雄性黄鳝随着性原的成熟其性腺蛋白组分则有所减少；；雌鱼性腺Ⅱ－Ⅲ期为１０－１２条区带，雄鱼性腺Ⅲ－Ⅵ期为１３－１０条区带。兼性期性腺蛋白组分明显增加为１５－１９条区带，其增加的蛋白带为一组位于凝胶偏负极端、分子量相近的蛋白分子，性逆转时精巢的组建可能与这组蛋白的调节有关。性逆     

雌核发育银鲫和两性融合发育鱼（红鲫和彩鲫）卵壳结构及其组成的比较研究

作者以两性融合发育鱼（红鲫、彩鲫）为对照,对雌核发育银鲫卵壳的表面结构及其可溶性蛋白的组成进行了研究：（１）雌核发育银鲫卵壳表面比较平滑,没有明显的嵴和沟;（２）雌核发育银鲫卵壳可溶性蛋白的含量略高于两性融合发育鱼（红鲫、彩鲫）,并且在ＩＩ区段存在一条分子量为１０万Ｄａｌｔｏｎ的特异蛋白区带。并对银鲫卵壳结构及组成的特殊性与银鲫卵初级控制作用间的关系进行了初步探讨。     

黄鳝血清和体表粘液蛋白的比较研究

本文用反相高效液相色谱法测定了黄鳝血清和体表粘液蛋白的氨基酸种类和含量,比较了二者的氨基酸组成变化。结果表明：二者都含有17种氨基酸,血清的氨基酸总量为397．11mg／l00ml,体表粘液蛋白的氨基酸总量为259．29mg／l00m1,血清与粘液蛋白中氨基酸含量差异最大的是蛋氨酸、半胱氨酸。应用SDS—PAGE分析和比较了血清和体表粘液蛋白的分子量大小及特有区带效,黄鳝血清与体表粘液蛋白分子量相同的蛋白区带数为2条,其分子量大小分别为19．5kDa、96．0kDa。其中血清的特有蛋白带为18条,体表粘液的特有蛋白带为8条。此外,对二者的相关性和体表粘液特异性的免疫机制作了探讨。     

大熊猫乳汁蛋白组成

测定了2只大熊猫（ailuropoda melanoleuca)乳汁中蛋白含量,乳糖含量,乳蛋白组成,并与成都麻羊（Capra hircus)初乳和中国荷斯坦牛（Bos taurus)乳进行了比较,大熊猫乳蛋白含量平均为41．52g/L,与中国荷斯坦牛乳接近;乳糖平均含量为15．41g/L,极显著低于牛乳和成都麻羊初乳,乳蛋白SDS－PAGE分析表明,大熊猫乳中酪蛋白（CN）含量明显低于羊乳和牛乳;乳中存在3条蛋白含量的区带,而在成都麻羊和中国荷斯坦牛乳电泳图谱的相应位置未见明显的区带,乳中上皮粘蛋白MUC1仅存在1条分子量约为196kDa的区带,未发现多态现象。     

牛脑中神经特异性S-100蛋白的纯化及鉴定

牛脑充分匀浆后经三次硫酸铵分级沉淀,再通过一次DEAE-Sepharose CL-6B层析柱,线性梯度洗脱后共收集4个峰洗脱液。PAGE分析(7.5％凝胶)显示第3峰为单一区带;免疫双扩散证实该洗脱液中蛋白为S-100蛋白。SDS-PAG E分析显示S-100蛋白分子量约为10kD;非还原条件下,凝胶过滤(Sephadex G-75)显示S-100蛋白位于MW为20kD区域。认为该纯化方法简便、快速,可获得较高纯度的S-100蛋白,活性高达1∶128以上,完全能满足进一步研究之用。     

抗胃癌单克隆抗体3H11对应抗原的纯化及鉴定

抗胃癌单克隆抗体3H11的对应抗原主要表达于靶细胞的膜上,不耐热,经蛋白酶消化,抗原失活。过碘酸氧化不影响活性,Schiff′s试剂糖柒色为阴性。SDS-PAGE显示单一区带,分子量为210kD。靶细胞经衣霉素抑制糖基化作用后,对其分子量无明显影响。等电聚焦电泳表明其等电点为8.5,故3H11抗原为一大分子碱性蛋白。     

霍乱弧菌EL－Tor35A3菌株外膜蛋白主区带的纯化

选用霍乱弧菌ＥＬ－Ｔｏｒ生物型３５Ａ３菌株（血清稻叶型）以ＥＤＴＡ－溶菌酶法与超速离心法提取其外膜蛋白,并将聚丙烯酰胺凝胶电泳后一条蛋白主区带分离。ＳＤＳ－聚丙烯酰胺凝胶电泳测得该蛋白主区带的分子量为２５ｋＤ,免疫电泳显示一条线,免疫双扩试验表明,不同的霍乱弧菌菌株均有该蛋白抗原存在。     

BAX敲除对小鼠大脑皮层和海马星形胶质细胞分布的影响

星形胶质细胞是大脑中一类高度异质的重要大胶质细胞,不仅在脑的发育和功能中起到重要作用,也参与多种神经病理生理学过程。多项研究表明B淋巴细胞瘤-2相关X蛋白(B-cell lymphoma-2 associated X protein,BAX)依赖性凋亡通路参与调控正常发育过程中脑内神经元的数量与分布,但是对其调控星形胶质细胞的研究则较为匮乏。本文旨在研究BAX是否参与不同脑区星形胶质细胞分布的调控。以纯合子和杂合子BAX敲除小鼠为研究对象,用SOX9免疫荧光染色法检测6周龄小鼠的大脑皮层和海马中星形胶质细胞的密度。结果显示,星形胶质细胞的密度在不同皮层分区之间以及皮层和海马之间存在显著差异,并且BAX敲除导致海马中星形胶质细胞的密度显著降低,皮层中GABA能抑制神经元密度显著升高,而皮层中星形胶质细胞的密度则未受显著影响。以上结果提示,BAX差异调控皮层星形胶质细胞与神经元,也差异调控皮层与海马中的星形胶质细胞。这项研究为了解星形胶质细胞的区域异质性和BAX在大脑发育中的功能提供了重要信息。     

Chromatin proteins associated with micrococcal nuclease-sensitive and nuclease-resistant chromatin fractions of Kirkman-Robbins hepatoma and hamster liver

Micrococcal nuclease-sensitive (SP) and nuclease-resistant (PP) chromatin fractions from Kirkman-Robbins hepatoma and hamster liver were obtained. The molecular distribution of three non-histone proteins (NHCP1, NHCP2 and NHCP3), histones, and chromatin-bound protease activity between SP and PP fractions of both tissues was compared. Differences, mainly of quantitative nature, among non-histone proteins of neoplastic and normal tissue were observed. Moreover, it was found that polypeptides with mol. wt 81 000 (NHCP1), 39 000 (NHCP2) and 21 000, 35 000, 37 000 (NHCP1), 70 000, 112 000, 141 000, 157 000 (NHCP2), 30 000–33 000 (NHCP3) were associated only with the nuclease-sensitive part of chromatin of hepatoma and normal tissue, respectively. A major difference in histone compostion of hamster hepatoma and liver concerns histones H2A and H1. Furthermore, an enrichment of high mobility group proteins as well as other soluble non-histone proteins in an acid extract of the SP fraction was observed. Apparently chromatin-bound protease activity can be found in both fractions of chromatin.     

NON-HISTONE CHROMOSOMAL PROTEINS IN MOUSE BRAIN AT DIFFERENT STAGES OF DEVELOPMENT AND IN A TRANSPLANTABLE MOUSE TERATOMA

Abstract— Non-histone chromosomal proteins (NHCP) from mouse brain at different stages of development and from adult liver and kidney of strain related mice were analyzed by SDS-polyacrylamide gel electrophoresis and were compared with the mouse teratoma, OTT-6050. The fetal, neonatal and adult brains were qualitatively similar in their NHCP profiles but had quantitative differences. The NHCP composition of the adult brain was clearly distinct from that of the liver and kidney and was dissimilar from that of the teratoma.     

Molecular characterization of non-histone chromatin proteins from experimental tumours

Using two-dimensional (2-D) electrophoresis, two non-histone chromatin protein fractions (NHCP1 and NHCP2) from three animal tumours (Kirkman-Robbins hepatoma, Morris hepatoma 7777 and Ehrlich ascites cells) and normal hamster liver were analyzed. Apart from many common components several tissue specific polypeptides of the NHCP1 and NHCP2 fractions were detected. It was found that some spots present in electropherograms of non-histone proteins of tumour cells (M X 10(-3)/pI): 17-24/4.9-6.5 (NHCP1 and NHCP2); 34-41/4.9-6.0 (HCP1 and NHCP2); 44-46/5.3-7.5 (HCP2); 46-49/5.0-7.5 (NHCP1); 49/5.9-7.5 (NHCP2) and 102-134/5.6-7.0 (NHCP1) were absent from normal liver.     

Cellular distribution of the hamster liver specific nucleolar antigens

The immunochemical localization of hamster liver nucleolar antigens in subcellular fractions (nuclei, 10,000 x g pellet, 100,000 x g pellet and supernatant), nuclear substructures (chromatin, nuclear matrix, nuclear envelope, nucleoli, RNP particles and nucleosomes), and three classes of nonhistone chromosomal proteins with different affinities to DNA (NHCP1, NHCP2 and NHCP3) from nuclease-sensitive and nuclease-resistant chromatin fractions of hamster liver were studied. Six main nucleolar antigens with mol. wts 27,000; 29,000; 30,000; 36,000; 45,000; and 46,000 were found in subcellular fractions, nuclear substructures and classes of non-histone proteins of hamster liver. The antigens with mol.wts of approx. 27,000; 29,000; and 36,000 which were absent in hamster pancreas, spleen and Kirkman--Robbins hepatoma nuclei, seem specific for liver tissue.     

Identification of protein kinase C and its potential substrate in Entamoeba histolytica

1. Protein kinase C (PKC) activity has been identified in various strains of the human parasite, Entamoeba histolytica. 2. An amoebic protein of mol. wt 78,000 was recognized by polyclonal antibodies raised against the 82,000 mol. wt rat brain protein kinase C. 3. A partially purified PKC preparation from E. histolytica phosphorylated histone I in the presence of calcium, phospholipids and diacylglycerol, and specifically bound tritiated phorbol ester at an apparent KD of 9 nM. 4. A relocalization of the amoebic PKC activity from the cytosol to the membrane fraction was observed when trophozoites were actively phagocytising bacteria. Under these conditions, a labelled phosphoprotein of mol. wt 68,000 was identified. 5. Similar to what was found during macrophage activation, a myristoylated mol. wt 68,000 protein was detected in amoebae grown in the absence of bacteria, but not in amoebae which were active in phagocytosis.     

Two types of receptor for insulin-like growth factors in mammalian brain.

Two types of receptor for insulin-like growth factors (IGFs) have been identified on adult rat and human brain plasma membranes by competitive binding assay, affinity labelling, receptor phosphorylation and interaction with antibodies to insulin receptors. The type I IGF receptor consists of two species of subunits: alpha-subunits (mol. wt. approximately 115 000), which bind IGF I and IGF II with almost equal affinity and beta-subunits (mol. wt. approximately 94 000), the phosphorylation of which is stimulated by IGFs. The alpha-subunits of type I IGF receptors in brain and other tissues differ significantly (mol. wt. approximately 115 000 versus 130 000), whereas the beta-subunits are identical (mol. wt. approximately 94 000). The type II IGF receptor in brain is a monomer (mol. wt. approximately 250 000) like that in other tissues. Two antibodies to insulin receptors, B2 and B9, interact with type I but not with type II IGF receptors. B2 is more potent than B9 in inhibiting IGF binding and in immunoprecipitating type I IGF receptors, in contrast to their almost equal effects on insulin receptors. This pattern is characteristic for IGF receptors in other cells. The presence of two types of IGF receptor in mammalian brain suggests a physiological role of IGFs in regulation of nerve cell function and growth. Since IGF II, but not IGF I, is present in human brain, we propose that IGF II interacts with both types of IGF receptor to induce its biological actions.     

Growth-related changes of non-histone chromatin proteins from Kirkman-Robbins hepatoma

1. Non-histone chromatin protein fractions NHCP1 and NHCP2 eluted from hydroxyapatite with 50 and 100 mM phosphate buffer (pH 6.8) from nuclei of Kirkman-Robbins hepatoma from 4th, 7th and 9th day of growth were analysed by one- and two-dimensional gel electrophoresis as well as Western blot technique in the presence of antibodies elicited against NHCP1, NHCP2 and dehistonized chromatin of hamster hepatoma and liver. 2. The presence of electrophoretically and immunologically specific components among NHCP1 and NHCP2 fractions during Kirkman-Robbins hepatoma growth was stated.     

Metabolic stability of nonhistone chromosomal proteins in two different classes of developing rat brain nuclei.

The metabolic behaviour of NHCP was studied in rat brain nuclei from fully differetiated cells and in nuclei from still differentiating cells. Eight-day-old rats were injected intracisternally with [14C]thymidine and [3H]tryptophan and the 3H/14C ratio of the chromatin was followed for a period of 33 days. It was found that in the fraction of differentiated cells this ratio remained unchanged, showing the presence of metabolically stable NHCP. At the same time in the fraction containing nondifferentiated cells a substantial part of the NHCP was turned over, which was indicated by a sharp decrease in their 3H/14C ratio with time.