Characterization of AT2 Receptor Expression in NIH 3T3 Fibroblasts

1. A high expression of angiotensin II receptors and of angiotensin-converting enzyme (ACE) activity was detected in confluent NIH 3T3 fibroblasts.2. Characterization with selective ligands, dithiothreitol, and GTPS, indicated that only the AT₂ subtype was expressed.3. AT₂ receptors and ACE expression were strictly dependent on the cell density and growth phase of the cells, with AT₂ receptors being expressed earlier than ACE. In contrast, high expression of AT₂ receptors irrespective of their growth state was observed in NIH 3T3 cells lacking contact inhibition upon neoplastic transformation with ras.4. Our results imply a possible relation of AT₂ receptors to cell growth and cell–cell contact.     

利用自裂解多肽T2A在牛耳皮肤成纤维细胞中实现多基因共同表达

目的:探讨利用自裂解多肽2A构建的多顺反子载体能否在牛耳皮肤成纤维细胞中实现多基因的有效表达。方法:利用来自一点褐翅蛾病毒(TaV)的2A元件(T2A)将GFP和Neo基因连接到同一载体中,构建pCMV-GFP-T2A-Neo质粒,将其转染牛耳皮肤成纤维细胞,以FACS检测GFP基因的表达,RT-qPCR检测GFP、T2A和Neo的表达。结果:由T2A连接的GFP和Neo基因在mRNA水平上都有显著表达,且表达水平相当。结论:以T2A连接的基因在转入细胞后能正常翻译和表达,显示T2A在牛耳皮肤成纤维细胞中具有自裂解功能,可作为一种构建多顺反子载体的有效工具用于牛耳皮肤成纤维细胞的基因转移,为其将来在转基因牛研制中的应用奠定了基础。     

Disruption of the Myostatin Gene in Porcine Primary Fibroblasts and Embryos Using Zinc-Finger Nucleases

Myostatin represses muscle growth by negatively regulating the number and size of muscle fibers. Myostatin loss-of-function can result in the double-muscling phenotype and increased muscle mass. Thus, knockout of myostatin gene could improve the quality of meat from mammals. In the present study, zinc finger nucleases, a useful tool for generating gene knockout animals, were designed to target exon 1 of the myostatin gene. The designed ZFNs were introduced into porcine primary fibroblasts and early implantation embryos via electroporation and microinjection, respectively. Mutations around the ZFNs target site were detected in both primary fibroblasts and blastocysts. The proportion of mutant fibroblast cells and blastocyst was 4.81% and 5.31%, respectively. Thus, ZFNs can be used to knockout myostatin in porcine primary fibroblasts and early implantation embryos.     

利用瞬间表达技术分析小麦抗病相关基因的功能

采用瞬间表达技术分析了TaTBL、TaPK1和TaTST等3个抗病相关基因的功能。首先将这3个小麦抗病相关基因构建入高效表达载体,然后使用基因枪将目标基因和GUS基因载体同时导入到感白粉病小麦品种离体叶片表皮细胞中,用GUS基因标记阳性转化细胞。转化后接种白粉菌孢子,48h后观察转化阳性表皮细胞,研究抗病相关基因表达对白粉菌入侵及吸器形成产生的影响。结果表明,这3个基因在感病小麦品种叶片表皮细胞中的瞬间表达,对白粉菌侵入和吸器形成均有部分抑制作用,在一定程度上增强了表达细胞对白粉菌的抗性。     

A New Method of Defense Response Analysis Using a Transient Expression System in Rice Protoplasts

We established a new plant defense response assay using a transient expression system in rice protoplasts. The assay system sensitively detected defense induction by flagellin, which had previously been assigned to a specific elicitor. Our assay system provides a rapid and efficient way to dissect rice defense mechanisms.     

草莓APETALA2同源基因的克隆及表达分析

利用同源克隆方法首次从草莓花芽cDNA中分离出APETALA2同源基因SAP2。SAP2全长182bp,编码435个氨基酸。序列分析表明,SAP2具有AP2家族典型的结构域。采用RT-PCR方法分析SAP2在不同组织中的表达情况,结果显示SAP2在草莓营养组织、花芽以及不同花器官中均有表达,与拟南芥AP2、矮牵牛PhAP2A的表达模式一致。以上结果说明SAP2是草莓的AP2同源基因。     

人管家基因启动子序列中的组合转录调控元件分析

研究表明,第一内含子可能参与基因转录调控.利用统计方法提取人管家基因上游至第一内含子序列中潜在的组合转录调控模体,分析模体间的距离、区域分布等特征,探讨内含子参与基因转录调控的可能性及其参与方式.在管家基因中共获得960对潜在转录调控模体对,其中57%与实验已知的具有转录相互作用的因子对吻合,共涉及12组因子对.分析发现,绝大多数模体对(80%)偏向于上游区域及"上游-内含子"区域,进一步支持了内含子参与基因转录调控的假设,并据此推测内含子与上游序列之间具有转录协同作用,模体在基因转录起始位点(TSS)附近较为集中,模体对的两个模体之间距离较近,60%左右距离在200 bp以内,特别地,65%的模体对特征距离在100 bp以内,短距离间隔有利于转录因子间的协同作用.这些结果将有助于对人基因转录调控机制及内含子功能的深入认识.     

Investigation of Reference Genes in Vibrio parahaemolyticus for Gene Expression Analysis Using Quantitative RT-PCR

Vibrio parahaemolyticus is a significant human pathogen capable of causing foodborne gastroenteritis associated with the consumption of contaminated raw or undercooked seafood. Quantitative RT-PCR (qRT-PCR) is a useful tool for studying gene expression in V. parahaemolyticus to characterize its virulence factors and understand the effect of environmental conditions on its pathogenicity. However, there is not a stable gene in V. parahaemolyticus that has been identified for use as a reference gene for qRT-PCR. This study evaluated the stability of 6 reference genes (16S rRNA, recA, rpoS, pvsA, pvuA, and gapdh) in 5 V. parahaemolyticus strains (O3:K6-clinical strain-tdh ⁺, ATCC33846-tdh ⁺, ATCC33847-tdh ⁺, ATCC17802-trh ⁺, and F13-environmental strain-tdh ⁺) cultured at 4 different temperatures (15, 25, 37 and 42°C). Stability values were calculated using GeNorm, NormFinder, BestKeeper, and Delta CT algorithms. The results indicated that recA was the most stably expressed gene in the V. parahaemolyticus strains cultured at different temperatures. This study examined multiple V. parahaemolyticus strains and growth temperatures, hence the finding provided stronger evidence that recA can be used as a reference gene for gene expression studies in V. parahaemolyticus.     

Analysis of K-Ras Nuclear Expression in Fibroblasts and Mesangial Cells

Background

Ras GTPases are considered cytoplasmic proteins that must be localized to cell membranes for activation, and there are few evidences of the presence of any Ras isoform in nuclei of eukaryotic cells.

Methodology/Principal Findings

Using conventional antibodies and inmunocytochemistry, differential centrifugation and western blot, we have observed the putative presence of K-Ras isoform in the nuclei of fibroblasts and mesangial cells. In order to avoid cross-reactions with other Ras isoforms, and using antibodies against K-Ras (R-3400, H3845-M01, sc-30) or pan-Ras (05-516, OP40) in cells that only expressed the K-Ras isoform (fibroblasts obtained from H-ras^−/−,N-ras^−/− mice) we also detected some nuclear positive expression. To further probe the identity of nuclear K-Ras, we have generated K-Ras knockout (K-ras^−/−) embrionary fibroblasts by mating of K-ras^+/− heterozygote mice. Using specific antibodies, only H- and N-Ras isoforms were observed in the cytoplasm of K-ras^−/− fibroblasts. However, both K-Ras4A and K-Ras4B positive signals were detected by immunocytochemistry and Western blot with two commercial antibodies (sc-522 and sc-521 against each isoforms, respectively) in both cytoplasm and nuclei from K-ras^−/− fibroblasts.

Conclusions/Significance

We show that the presence of K-Ras4B in fibroblast nuclei, already described by other authors, is probably due to a cross-reaction of the antibody with an undetermined nucleolar protein. Although this study also shows the possible nuclear expression of K-Ras isoform in fibroblasts or in mesangial cells, it also reveals the importance of being cautious in these studies about distribution of protein isoforms due to some important limitations imposed by the unspecificity of the antibodies or contaminations in cellular preparations.     

MouseSprr2Genes: A Clustered Family of Genes Showing Differential Expression in Epithelial Tissues

Small proline-rich (SPR) proteins are structural components of the cornified cell envelope of stratified squamous epithelia. They are subdivided into three families, i.e., SPR1, SPR2, and SPR3, of which the SPR2 family is the most complex. To understand the significance of this complexity, we have isolated 11 mouseSprr2genes, constructed a provisional physical map of theSprr2locus on mouse Chromosome 3, and examined the expression patterns of theSprr2genes in mouse epithelial tissues. The 11Sprr2sequences are highly conserved with a central domain containing a variable number of repeats.In situhybridization showed theSprr2expression to be confined to epithelia. RT-PCR using primers specific for each of the 11Sprr2members demonstrated varying degrees of expression among the individualSprr2members in different tissues. The correlation between the physical location of the genes in theSprr2locus and their expression patterns suggests multiple levels of controlled expression.     

Expression of Discoidin Domain Receptor 2 (DDR2) Extracellular Domain in Pichia Pastoris and Functional Analysis in Synovial Fibroblasts and NIT3T3 Cells

Discoidin domain receptor 2 (DDR2) is a kind of protein tyrosine kinases associated with cell proliferation and tumor metastasis, and collagen, identified as a ligand for DDR2, up-regulates matrix metallloproteinase 1 (MMP-1) and MMP-2 expression in cellular matrix. To investigate the roles of DDR2 in destruction of cartilage in rheumatoid arthritis (RA) and tumor metastasis, we tried to express extracellular domain of DDR2 fused with a His tag to increase protein solubility and facilitate purification (without signal peptide and transmembrane domain, designated DR) in Pichia pastoris, purify the expressed protein, and characterize its function, for purpose of future application as a specific DDR2 antagonist. Two clones of relative high expression of His-DR were obtained, After purification by a Ni-NTA (nitric-tri-acetic acid) chromatographic column, soluble fused His-DR over 90% purity were obtained. Competitive binding inhibition assay demonstrated that expressed His-DR could block the binding of DDR2 and natural DDR2 receptors on NIT3T3 and synovial cell surfaces. Results of RT-PCR, Western blotting, and gelatinase zymography showed that His-DR was capable of inhibiting MMP-1 and MMP-2 secretion from NIT3T3 cells and RA synoviocytes stimulated by collagen II. For MMP-1, the inhibitory effect was displayed at the levels of mRNA and protein, whereas for MMP-2 it was demonstrated at the level of protein physiological activity. All these findings suggested that the fused expressed His-DR inhibited the activity of natural DDR2, and relevant MMP-1 and MMP-2 expression in synoviocytes and NIH3T3 cells provoked by collagen II. Wei Zhang and Tianbing Ding equally contributed to this work.     

Potency Analysis of Mesenchymal Stromal Cells Using a Combinatorial Assay Matrix Approach

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Identification of Novel Reference Genes Using Multiplatform Expression Data and Their Validation for Quantitative Gene Expression Analysis

Normalization of mRNA levels using endogenous reference genes (ERGs) is critical for an accurate comparison of gene expression between different samples. Despite the popularity of traditional ERGs (tERGs) such as GAPDH and ACTB, their expression variability in different tissues or disease status has been reported. Here, we first selected candidate housekeeping genes (HKGs) using human gene expression data from different platforms including EST, SAGE, and microarray, and 13 novel ERGs (nERGs) (ARL8B, CTBP1, CUL1, DIMT1L, FBXW2, GPBP1, LUC7L2, OAZ1, PAPOLA, SPG21, TRIM27, UBQLN1, ZNF207) were further identified from these HKGs. The mean coefficient variation (CV) values of nERGs were significantly lower than those of tERGs and the expression level of most nERGs was relatively lower than high expressing tERGs in all dataset. The higher expression stability and lower expression levels of most nERGs were validated in 108 human samples including formalin-fixed paraffin-embedded (FFPE) tissues, frozen tissues and cell lines, through quantitative real-time RT-PCR (qRT-PCR). Furthermore, the optimal number of nERGs required for accurate normalization was as few as two, while four genes were required when using tERGs in FFPE tissues. Most nERGs identified in this study should be better reference genes than tERGs, based on their higher expression stability and fewer numbers needed for normalization when multiple ERGs are required.     

猪生长激素基因在杆状病毒载体系统中的表达

通过对猪生长激素(pGH)基因的cDNA进行测序,得到pGH cDNA的全序列,并与Seeburg等报道的序列进行了比较和讨论.然后利用具人工合成启动子和多角体蛋白XIV启动子的转移载体质粒pSXIVVI+X3/4构建出含pGH基因的重组质粒pX3/4-pGH.将pX3/4-pGH与致死缺失型线性化AcMNPV-OCC- DNA共转染Sf9细胞,构建出既能形成多角体又能表达pGH基因的苜蓿丫纹夜蛾核多角体重组病毒AcMNPV-pX3/4-pGH-OCC+.感染重组毒株的Hi 5细胞可溶蛋白及其培养上清的SDS-PAGE和Western blot的分析结果表明,感染细胞的蛋白电泳带的20.7 kDa处有一条猪生长激素特异带,但培养上清中没有.凝胶黑度扫描估测结果显示pGH蛋白占细胞可溶蛋白的4.48%.