锌协同三羟异黄酮对成骨细胞MC3T3-E1的影响

目的:观察锌协同三羟异黄酮对成骨细胞MC3T3-E1增殖、细胞中碱性磷酸酶(ALP)含量、骨形成蛋白-2(BMP-2)表达的影响,探讨锌协同三羟异黄酮对骨质疏松的防治作用.方法:采用四甲基偶氮噻唑蓝比色法检测(1×10-7)mol/L、(1×10-6)mol/L、(1x 10-5)mol/L、(1×10-4)mol/L的三羟异黄酮以及与(1×10-5)mol/L锌联合作用时对MC3T3-E1增殖的作用;应用Western blot法检测三羟异黄酮与锌联合作用前后,成骨细胞中BMP-2蛋白的表达水平,用比色法检测MC3T3-E1中ALP的含量.结果:锌与三羟异黄酮单独作用或协同作用于MC3T3-E1细胞,其增殖率随着三羟异黄酮浓度的增加和作用时间的延长而升高,(1×10-5)mol/L的三羟异黄酮协同(1×10-5)mol/L的锌作用72h,其细胞增殖率为(160.1±14.3)%.细胞中的LP含量及BMP-2的表达也随着三羟异黄酮浓度的增加及作用时间的延长而增加.三羟异黄酮和锌联合作用后,对ALP活性的增强、BMP-2表达的增加作用均较各自单独作用时更为明显(P＜0.05).结论:三羟异黄酮与锌协同作用表现出雌激素效应,可通过促进骨形成蛋白的合成从而促进成骨细胞的增殖、增加骨量.     

肿瘤坏死因子α对ROS17/2.8细胞甲状旁腺素受体的下行调节

肿瘤坏死因子α(TNFα)是激活的单核巨噬细胞分泌的蛋白质,分子量17kD。其多功能性和选择性抑制肿瘤细胞生长的作用受到高度重视。我们的实验表明:TNFα(3×10~(-10)-1×10~(-7)mol/L)能显著降低大鼠成骨肉瘤细胞株ROS17/2.8的甲状旁腺素(PTH)受体总结合率,比对照降低7.47-37.45％,且与TNFα的浓度呈正相关。时间曲线显示,TNFα作用时间越长,受体总结合率降低越明显。Scatchard作图表明PTH受体数目降低而其亲和力无显著变化。细胞周期分析显示,TNFα(3.83×10~(-10) mol/L作用3天)能抑制S期DNA合成。可见TNFα通过减少PTH受体数目以调节骨代谢。同时通过抑制DNA的合成以调节骨细胞的增殖。     

补骨脂素对中波紫外线导致人皮肤HaCaT细胞光老化的保护作用

目的:研究补骨脂素对中波紫外线(UVB)导致人皮肤HaCaT细胞光老化的保护作用及其作用机制。方法:选择不同浓度的补骨脂素,MTT法筛选药物的浓度;使用中波紫外线(UVB)照射永生化的HaCaT细胞建立UVB光老化模型;使用三种不同浓度的补骨脂素处理光老化模型,MTT法检测细胞的增殖及氧化试剂盒检测细胞中氧化酶的活性。RT-PCR及Western Blot分别检测JNK和白介素-8(IL-8)mRNA及蛋白表达量。结果:与空白组相比,10~(-7)mol/L、10~(-6)mol/L、10~(-5)mol/L补骨脂素组对HaCaT具有无明显的增殖作用(P0.05);与模型组相比,10~(-7)mol/L、10~(-6)mol/L、10~(-5)mol/L补骨脂素组对HaCaT具有无明显的增殖作用(P0.05),但是10~(-7)mol/L、10~(-6)mol/L、10~(-5)mol/L补骨脂素组SOD、GSH、CAT活性升高(P0.01),细胞JNK、IL-8 mRNA表达量均降低(P0.01),细胞JNK、IL-8蛋白表达量均降低(P0.05或P0.01)。结论:补骨脂素能够显著的保护HaCaT细胞的光老化,其机制可能与增强抗氧化酶活性,及抑制JNK信号通路,减少炎症因子的分泌有关。     

睾酮对内皮细胞妊娠相关血浆蛋白-A mRNA表达的影响

目的:观察睾酮对内皮细胞妊娠相关血浆蛋白-A(PAPP-A)m RNA表达的影响。方法:人原代脐静脉内皮细胞,选择第3~4代生长状态良好的细胞用于实验。实验分组:1空白对照组;2肿瘤坏死因子(TNF)-α(终浓度100μg/L)培养细胞组;3TNF-α(终浓度100μg/L)及睾酮1×10-8mol/L培养细胞组;4睾酮1×10-8mol/L培养细胞组。实验结束后收集各组细胞,用RT-PCR方法检测各组细胞PAPP-A m RNA表达水平。结果:TNF-α作用2 h后,内皮细胞中PAPP-A m RNA表达水平升高(P0.05),且随TNF-α作用时间的延长,PAPP-A表达逐渐升高,在16小时达高峰;睾酮作用后,PAPP-A m RNA表达水平较TNF-α组明显降低(P0.01)。结论:TNF-α上调内皮细胞PAPP-A m RNA的表达,而睾酮抑制了TNF-α对PAPP-A分泌增加的刺激作用。     

阿魏酸在缺氧条件下促进人脐静脉内皮细胞血管形成的实验研究

目的:研究阿魏酸(ferulic acid,FA)在缺氧条件下对人脐静脉内皮细胞(human umbilical vein endothelial cells,HUVECs)增殖、迁移和管腔样结构形成的影响。方法:原代培养人脐静脉内皮细胞,在缺氧实验条件下,细胞被分为7组,即1个对照组和6个实验组。对照组采用1%酒精处理,实验组用不同浓度(1×10~(-8)、1×10~(-7)、1×10~(-6)、1×10~(-5)、1×10~(-4)及1×10~(-3) mol/L)的阿魏酸处理。分别采用MTS法、划痕法、Matrigel法分析不同浓度阿魏酸处理对人脐静脉内皮细胞的增殖、迁移和管腔样结构形成的影响。结果:缺氧条件下,浓度为1×10~(-6)~1×10~(-4)mol/L的阿魏酸处理能明显促进HUVECs的增殖(P0.05),以1×10~(-5) mol/L处理的效果最好(P0.01);与对照组相比,1×10~(-6)mol/L(P0.05)、1×10~(-5) mol/L(P0.01)及1×10~(-4) mol/L(P0.01)阿魏酸处理均能明显促进HUVECs横向迁移,以1×10~(-5) mol/L处理迁移的细胞数量最多;1×10~(-8)~1×10~(-4) mol/L阿魏酸处理能不同程度地促进HUVECs管腔样结构的形成,以1×10~(-5) mol/L处理形成管腔样结构的数量最多(P0.01)。结论:阿魏酸在缺氧条件下能促进人脐静脉内皮细胞的增殖、迁移和管腔样结构形成。     

高糖诱导肾小球系膜细胞表达TNFα-的机制探讨

目的:初步探讨高糖诱导肾小球系膜细胞表达肿瘤坏死因子α(TNFα-)的机制。方法:分别用p38丝裂原活化蛋白激酶(p38MAPK)特异性抑制剂SB203580、核因子-κB(NFκ-B)特异性抑制剂PDTC预刺激肾小球系膜细胞30 min,再以高糖(20 mmol/L)干预48 h后,分别采用RT-PCR法检测系膜细胞内TNFα-mRNA水平,Western blot法检测系膜细胞内磷酸化p38MAPK蛋白水平、细胞核及细胞浆NFκ-B p65蛋白水平。结果:与低糖对照组相比,高糖可促进肾小球系膜细胞内TNFα-mRNA表达,以及p38MAPK、NFκ-B蛋白活化;SB203580(10 mmol/L)、PDTC(10 mmol/L)预刺激肾小球系膜细胞均可抑制高糖诱导肾小球系膜细胞表达TNFα-,且SB203580可抑制高糖诱导系膜细胞内NFκ-B蛋白活化。结论:p38MAPK-NFκ-B信号途径参与介导高糖诱导肾小球系膜细胞表达TNFα-。     

地塞米松对TRAIL双向诱导猪肾成纤维细胞增殖与凋亡作用的影响

采用MTT掺入法检测细胞活率变化,分别筛选出诱导细胞增殖与凋亡的药物浓度;半定量PCR法检测不同浓度下地塞米松对骨保护素(Osteoprotegerin,OPG)和核因子κB受体激活剂受体配体(Ligand of receptor activator of nuclear factor kappa B,RANKL)基因在mRNA水平上的调控作用;流式细胞术检测细胞周期分布和凋亡率变化,显微镜观察FRSs存活、增殖和凋亡变化.经MTT检测和浓度筛选,发现TRAIL在0.01-5 mg/L浓度范围内诱导FRSs增殖,浓度增加到10 mg/L出现凋亡趋势.地塞米松可协同TRAIL双向诱导FRSs增殖或凋亡,有效浓度约10-6-10-10 mol/L.细胞周期分析与凋亡率检测结果表明RAIL诱导FRSs增殖峰浓度为5 mg/L.TRAIL(5 mg/L)与地塞米松协同作用,细胞增殖指数(Prl.)较TRAIL5 mg/L组上升2.49%(P<0.05);TRAIL 10 mg/L组与空白对照组比较细胞增殖指数和凋亡率无显著变化,TRAIL 10 mg/L与地塞米松协同作用G0/G1期比例较TRAIL10 mg/L组增加2.36%(P<0.05),凋亡率较之上升6.79%(P<0.01).地塞米松作用下,OPG基因mRNA水平表现下调,RANKL基因则表现上调,二者均表现为剂量依赖型.综上所述,TRAIL对FRSs呈诱导增殖或凋亡的双向调控作用,并呈剂量依赖型.地塞米松可协同TRAIL对FRSs作用,该现象与TRAIL和地塞米松诱导FRSs细胞周期的改变以及地塞米松对OPG/RANK/RANKL信号通路的OPG和RANKL基因的表达调控相关.     

细胞因子对鸡胚胎原始生殖细胞（EPGCs）增殖的影响

采用MTT法分别检测mLIF、bFGF、hSCF、hIL-11四种细胞因子协同作用对体外培养的第19、28期鸡EPGCs生长的影响。结果表明：与对照组相比较,19期的EPGCs体外培养72h后, mLIF、hSCF、bFGF、hIL-11对鸡EPGCs的增殖影响显著（P<0.05）。mLIF的最佳作用剂量是10~20ng/ml,hSCF的最佳作用剂量是15~20ng/ml,bFGF的最佳作用剂量是10～20ng/ml。hSCF、bFGF的联合使用优于单因子作用的结果（P<0.05）。单独使用hIL-11时,细胞的增殖情况比其他三因子单独使用的效果较差,但OD均值有随剂量增高而上升的趋势。在与其他因子联合使用的情况下, hIL-11的最佳作用剂量为0.10~0.20ng/ml。     

HSV体外感染对IgG产生的抑制作用和TNF及r-IFN对它的影响

本文观察了体外HSV-I感染对人淋巴细胞增殖、分化,产生免疫球蛋白的影响。HSV-I能感染PWM刺激的人扁桃体淋巴细胞,并抑制其增殖和免疫球蛋白(IgG)的产生,感染实验组的IgG产量较对照组明显降低(P<0.005)。HSV-I感染后,上清中可检出一定量的病毒,其滴度为10~(3·2)—10~(5·7)TCID50/ml;直接免疫荧光法检出病毒抗原阳性细胞为3％—8.5％。在感染实验系统中加入重组的IFN_a(r-IFN_a)、IFN_γ(r-IFN_γ)和纯化的肿瘤坏死因子(TNF),观察到r-IFN。和TNF均有一定程度抗病毒作用,部分解除HSV-I对IgG产生的抑制作用。和对照组相比,差异显著(P<0.01)。r-IFN_γ对HSV-I的感染和IgG产生几乎无作用(P>0.05),但r-IFN_γ对TNF有协同作用:抑制病毒增殖和解除HSV-I对IgG产生的抑制,比单独用TNF组更为显著(P<0.01)。     

多囊蛋白-1氨基段融合蛋白对大鼠肾小球系膜细胞周期及其调控基因表达的影响

研究多囊蛋白-1氨基段(PC-1NF)融合蛋白对大鼠肾小球系膜细胞(MC)周期及其调控基因表达的影响。应用Brdu-ELISA法检测PC-1NF融合蛋白对MC增殖的作用,流式细胞术观察PC-1NF融合蛋白对MC周期的影响,实时荧光定量RT-PCR方法检测PC-1NF融合蛋白对MC周期调控基因cyclinD1、p21WAF1表达的作用。结果表明PC-1NF融合蛋白能抑制MC增殖,呈现良好的时效与量效关系;PC-1NF融合蛋白能影响MC周期,使G0/G1期细胞增加,S期细胞减少;4μg/mlPC-1NF融合蛋白作用后,cyclinD1mRNA水平比对照组明显下调(P<0.05);而p21WAF1mRNA水平比对照组显著上调(P<0.01)。PC-1NF融合蛋白能抑制MC增殖及周期的进展,其机制可能是通过下调cyclinD1、上调p21WAF1的表达,抑制细胞通过G1-S调控点而介导的。     

Cell separation with horizontal cell electrophoresis under near-isopycnic conditions on a “density cushion”

This report describes an improvement made to the horizontal cell electrophoresis methodology. It involves using two liquid layers differing in density to produce an interface described as a "density cushion". The electrophoretic system that employed an anti-convective porous matrix to separate red blood cells (RBC) and charged dyes effectively was found to be unsuitable for some other mammalian cells. The "density cushion" method was found to be more versatile and applicable to studies on the separation of a variety of cell types. The experiments described show the differences between the electrophoretic mobilities of a human eosinophilic leukaemia cell line (Eol-1) and RBC, both with and without the modification of the cell surface properties.     

Cell electrophoresis — a method for cell separation and research into cell surface properties

In this paper, we discuss the application of various methods of cell electrophoresis in research into cell surface properties (analytical methods), and the separation of uniform cell subpopulations from cell mixtures (preparative methods). The emphasis is on the prospects of the development of simplified and versatile methodologies, i.e. microcapillary cell electrophoresis and horizontal cell electrophoresis under near-isopycnic conditions. New perspectives are considered on the use of analytical and preparative cell electrophoresis in research on cell differentiation, neoplastic transformation, cell-cell interactions and the biology of stem cells. Paper authored by participants of the international conference: XXXIV Winter School of the Faculty of Biochemistry, Biophysics and Biotechnology of Jagiellonian University, Zakopane, March 7–11, 2007, “The Cell and Its Environment”. Publication cost was covered by the organisers of this meeting.     

Polarization and Migration of Hematopoietic Stem and Progenitor Cells Rely on the RhoA/ROCK I Pathway and an Active Reorganization of the Microtubule Network

Understanding the physiological migration of hematopoietic progenitors is important, not only for basic stem cell research, but also in view of their therapeutic relevance. Here, we investigated the role of the Rho kinase pathway in the morphology and migration of hematopoietic progenitors using an ex vivo co-culture consisting of human primary CD34⁺ progenitors and mesenchymal stromal cells. The addition of the Rho kinase inhibitor Y-27632 led to the abolishment of the uropod and microvillar-like structures of hematopoietic progenitors, concomitant with a redistribution of proteins found therein (prominin-1 and ezrin). Y-27632-treated cells displayed a deficiency in migration. Time-lapse video microscopy revealed impairment of the rear pole retraction. Interestingly, the knockdown of ROCK I, but not ROCK II, using RNA interference (RNAi) was sufficient to cause the referred morphological and migrational changes. Unexpectedly, the addition of nocodazole to either Y-27632- or ROCK I RNAi-treated cells could restore their polarized morphology and migration suggesting an active role for the microtubule network in tail retraction. Finally, we could demonstrate using RNAi that RhoA, the upstream regulator of ROCK, is involved in these processes. Collectively, our data provide new insights regarding the role of RhoA/ROCK I and the microtubules in the migration of stem cells.     

酸性磷酸酶法检测体外培养细胞数

利用小鼠成纤维细胞系(NIH3T3)、小鼠骨髓瘤细胞系(SP2/0)、人大肠癌细胞系(LO-VO)和人白血病细胞系(K562),评价酸性磷酸酶(APA)法用于检测体外各类型细胞的增殖和杀伤作用。用直线回归分析光吸收度与每孔活细胞数的关系。结果表明,APA法能准确地反映检测的活细胞数(相关系数均>0.99)。本方法不仅能很好地检测表皮生长因子对细胞的增殖作用,也能够检测顺铂对体外细胞的杀伤作用。结果表明APA法简单、灵敏,可以用于上皮和间质等贴壁和悬浮生长的细胞计数。     

Expanisns

Biochemical dissection of the “acid-growth” process of plant cell walls led to the isolation of a new class of wall loosening proteins, called expansins. These proteins affect the rheology of growing walls by permitting the microfibril-matrix network to slide, thereby enabling the wall to expand. Molecular sequence analysis suggests that expansins might have a cryptic glycosyl transferase activity, but biochemical results suggest that expansins disrupt noncovalent bonding between microfibrils and the matrix. Recent discoveries of a new expansin family and gene expression in fruit, meristerms and cotton fibers have enlarged our view of the developmental functions of this group of wall loosening proteins.     

犬皮肤成纤维细胞的分离、培养及鉴定

目的探索和建立适用于犬皮肤成纤维细胞的体外分离、培养及鉴定的技术方法。方法采用组织贴块培养法和胰蛋白酶、胶原酶Ⅰ联合消化法对犬皮肤成纤维细胞进行体外培养、传代。并对所培养的细胞进行倒置显微镜观察和苏木素-伊红染色,观察成纤维细胞形态,并对培养细胞行波形蛋白免疫荧光染色。结果倒置相差显微镜下可见长梭形细胞生长,苏木素-伊红染色可见细胞呈漩涡状、平行排列,第5代细胞免疫荧光检测波形蛋白(vimentin)表达阳性。结论建立了高效快速分离和稳定培养成纤维细胞的方法,为诱导犬心房纤维化提供了充足的种子细胞。     

An overview of the KIN1/PAR-1/MARK kinase family

Members of the KIN1/PAR-1/MARK kinase family are conserved from yeast to humans and share a similar primary structural organization. Several kinases of this family appear to be at the crossroads of various biological functions including cell polarity, cell cycle control, intracellular signalisation, microtubules stability and protein stability. Here we present an overview of known roles of KIN1/PAR-1/MARK kinases including pEg3 a newly identified member which is regulated during the cell cycle and is a potential regulator of the cell cycle progression. Some common modes of action can be deciphered for this protein kinase family.     

Molecular basis for T cell response induced by altered peptide ligand of type II collagen

Mounting evidence from animal models has demonstrated that alterations in peptide-MHC interactions with the T cell receptor (TCR) can lead to dramatically different T cell outcomes. We have developed an altered peptide ligand of type II collagen, referred to as A9, which differentially regulates TCR signaling in murine T cells leading to suppression of arthritis in the experimental model of collagen-induced arthritis. This study delineates the T cell signaling pathway used by T cells stimulated by the A9·I-A(q) complex. We have found that T cells activated by A9 bypass the requirement for Zap-70 and CD3-ζ and signal via FcRγ and Syk. Using collagen-specific T cell hybridomas engineered to overexpress either Syk, Zap-70, TCR-FcRγ, or CD3-ζ, we demonstrate that A9·I-A(q) preferentially activates FcRγ/Syk but not CD3-ζ/Zap-70. Moreover, a genetic absence of Syk or FcRγ significantly reduces the altered peptide ligand induction of the nuclear factor GATA3. By dissecting the molecular mechanism of A9-induced T cell signaling we have defined a new alternate pathway that is dependent upon FcRγ and Syk to secrete immunoregulatory cytokines. Given the interest in using Syk inhibitors to treat patients with rheumatoid arthritis, understanding this pathway may be critical for the proper application of this therapy.     

A Scalable Approach to Prevent Teratoma Formation of Human Embryonic Stem Cells

As the renewable source of all cell types in the body, human embryonic stem cells (hESCs) hold great promise for human cell therapy. However, one major bottleneck that hinders the clinic application of hESCs is that hESCs remaining with their differentiated derivatives pose cancer risk by forming teratomas after transplantation. NANOG is a critical pluripotency factor specifically expressed in hESCs but rarely in their differentiated derivatives. By introducing a hyperactive variant of herpes simplex virus thymidine kinase gene into the 3′-untranslated region of the endogenous NANOG gene of hESCs through homologous recombination, we developed a safe and highly scalable approach to efficiently eliminate the teratoma risk associated with hESCs without apparent negative impact on their differentiated cell types. As thymidine kinase is widely used in human gene therapy trials and is the therapeutic target of U. S. Food and Drug Administration-approved drugs, our strategy could be effectively applied to the clinic development of hESC-based human cell therapy.     

The plant cell body: a cytoskeletal tool for cellular development and morphogenesis

Summary Certain aspects of cellular behaviour in relation to growth and development of plants can be understood in terms of the cell body concept proposed by Daniel Mazia in 1993. During the interphase of the mitotic cell cycle, the plant cell body is held to consist of a nucleus and a perinuclear microtubule-organizing centre from which microtubules radiate into the cytoplasm. During mitosis and cytokinesis in meristematic cells, and also during the period of growth in post-mitotic cells immediately beyond the meristem, the plant cell body undergoes various characteristic morphological transformations, many of which are proposed as being related to changing structural connections with the actin-based component of the cytoskeleton and with specialized, plasma-membrane-associated sites at the cell periphery. In post-mitotic cells, these transformations of the plant cell body coincide with, and probably provide conditions for, the various pathways of development which such cells follow. They are also responsible, for the acquisition of new cellular polarities. Events in which the plant cell body participates include the formation of a mitotic spindle, phragmoplast, and new cell division wall, the rearrangement of a diffuse type of cell wall growth into tip growth (as occurs, e.g., during the initiation and subsequent development of root hairs), and the growth and division that occurs in reactivated vacuolate cells. If more evidence can be marshalled in support of the existence and properties of the plant cell body, then this concept could prove useful in interpreting the cytological bases of a range of developmental events in plants.Abbreviations CMT cortical microtubule - EMT endoplasmic microtubule - ER endoplasmic reticulum - MF microfilament - MT microtubule - MTOC microtubule-organizing centre - PPB preprophase band (of microtubules) - QC quiescent centre - VSC vesicle supply centre