双委夜蛾气味结合蛋白AdisOBP6的原核表达抗体制备及表达谱分析

【目的】本研究旨在对双委夜蛾Athetis dissimilis气味结合蛋白OBP6进行原核表达、抗体制备以及表达谱分析,便于今后对AdisOBP6功能展开研究。【方法】利用生物信息学软件分析AdisOBP6蛋白结构特征;利用通过原核表达获得的重组蛋白4次免疫新西兰大白兔,制备AdisOBP6抗体;采用荧光定量PCR和Western blot技术检测AdisOBP6在双委夜蛾雌雄成虫触角、不同时期精巢以及受精卵和未受精卵中的表达情况。【结果】同源建模预测显示,AdisOBP6具有6个保守半胱氨酸残基和7个α-螺旋结构,并 折叠成一个结合口袋。原核表达结果显示,在20℃下0.5 mmol/L IPTG诱导重组蛋白表达量最多、最稳定。4次免疫重复中,抗体效价分别超过1∶512 000, 1∶512 000, 1∶512 000和1∶64 000。Westernblot检测获得的抗体与AdisOBP6蛋白能够特异性结合。荧光定量PCR结果显示,AdisOBP6在双委夜蛾精巢中的表达量远高于在触角中的,在幼虫期精巢中AdisOBP6就已经开始表达,在蛹期精巢中表达量低于在幼虫期的, 成虫羽化后精巢中的表达量逐渐进入高峰,在未受精卵和受精卵中几乎不表达或表达量极低。Western blot分析发现,AdisOBP6蛋白也主要在精巢中表达,在雌雄成虫触角、受精卵和未受精卵中表达量很低。【结论】本研究实现了AdisOBP6的原核表达,成功地制备了抗体;并证实AdisOBP6在双委夜蛾精巢中大量表达,成虫羽化后表达量达到高峰,推测AdisOBP6可能参与了授精过程。本研究结果为今后进一步研究AdisOBP6的功能奠定了基础。     

Rapid directed molecular evolution of fluorescent proteins in mammalian cells

In vivo imaging of model organisms is heavily reliant on fluorescent proteins with high intracellular brightness. Here we describe a practical method for rapid optimization of fluorescent proteins via directed molecular evolution in cultured mammalian cells. Using this method, we were able to perform screening of large gene libraries containing up to 2 × 10⁷ independent random genes of fluorescent proteins expressed in HEK cells, completing one iteration of directed evolution in a course of 8 days. We employed this approach to develop a set of green and near‐infrared fluorescent proteins with enhanced intracellular brightness. The developed near‐infrared fluorescent proteins demonstrated high performance for fluorescent labeling of neurons in culture and in vivo in model organisms such as Caenorhabditis elegans, Drosophila, zebrafish, and mice. Spectral properties of the optimized near‐infrared fluorescent proteins enabled crosstalk‐free multicolor imaging in combination with common green and red fluorescent proteins, as well as dual‐color near‐infrared fluorescence imaging. The described method has a great potential to be adopted by protein engineers due to its simplicity and practicality. We also believe that the new enhanced fluorescent proteins will find wide application for in vivo multicolor imaging of small model organisms.     

Menin regulates lipid deposition in mouse hepatocytes via interacting with transcription factor FoxO1

Molecular and Cellular Biochemistry - Non-alcoholic fatty liver disease (NAFLD) is rapidly being recognized as the leading cause of chronic liver disease worldwide. Men1, encoding protein of menin,...     

基于Cfku70基因失活策略构建果生刺盘孢的高效基因敲除底盘菌株

果生刺盘孢侵染危害多种植物,是重要的植物病原真菌。在一些丝状真菌中,敲除非同源末端连接修复通路的关键基因ku70或ku80可显著提高同源重组效率,进而提高靶基因置换频率。本研究从果生刺盘孢基因组鉴定到Cfku70和Cfku80两个基因,并明确了基因失活对菌株生物学表型和基因敲除效率的影响。敲除Cfku70或Cfku80不影响菌株的菌落形态、营养生长、产孢、分生孢子萌发、侵染结构发育和致病;Cfku70基因敲除还大幅提升3个测试基因的敲除效率。本研究证实Cfku70基因失活能显著提高果生刺盘孢的基因敲除效率,适宜作为高效基因敲除的底盘菌株,研究结果为通过批量敲除策略筛选新型致病因子奠定重要基础。     

果生刺盘孢效应蛋白CfEC92靶向Mal d 1j抑制苹果免疫

由果生刺盘孢引起的炭疽叶枯病是我国苹果产区的重要病害。果生刺盘孢在侵染苹果过程中分泌效应蛋白CfEC92促进其侵染,但其作用机制仍不清楚。本研究从苹果cDNA中克隆出Mal d 1j蛋白,结构域及氨基酸序列分析显示,Mal d 1j为PR10家族成员。Mal d 1j基因过表达能显著增强苹果对炭疽叶枯病抗性,而沉默Mal d 1j显著降低其抗性。在烟草中过表达Mal d 1j提高烟草抗性,共表达CfEC92和Mal d 1j蛋白,降低Mal d 1j对疫霉菌抗性。通过酵母双杂交、BIFC和Co-IP分析证明CfEC92与Mal d 1j可以发生直接互作,且其互作定位于细胞膜和细胞核,表明CfEC92 通过与Mal d 1j互作影响植物免疫。本研究揭示了果生刺盘孢效应蛋白CfEC92通过靶向Mal d 1j抑制植物免疫促进其侵染的分子机制,为苹果炭疽叶枯病防控提供了新的思路。     

A novel anti-DR5 chimeric antibody and epirubicin synergistically suppress tumor growth

Tumor necrosis factor-related apoptosis-inducing ligand (TRAIL) induces apoptosis in a variety of tumor cells. TRAIL receptor 2 (DR5) expression is high in tumor cells, transformed cells, and clinical tumor specimens and is low in most normal cells and tissues; therefore, DR5 is considered an attractive target for cancer therapy. In this study, HMCAZ5, a novel mouse-human chimeric antibody based on AD5-10, was generated and stably expressed in CHO-dhfr(-) cells. Highly purified HMCAZ5 exhibits a high affinity for the receptor that is equal to the parental mouse antibody, induces apoptosis in various cancer cells but not in normal hepatocytes, and elicits both antibody-dependent cellular cytotoxicity and complement-dependent cytotoxicity in various human cancer cells. The anthracycline anticancer drug epirubicin (EPB) synergizes the cytotoxicity of HMCAZ5 in cancer cells by upregulating DR5 expression on the cell surfaces, enhancing p53 expression, Bid cleavage, and JNK phosphorylation and downregulating c-FLIP expression and Akt phosphorylation. Moreover, HMCAZ5 alone suppresses tumor growth, and EPB augments the tumoricidal activity in human colorectal and hepatocellular tumor xenografts in athymic nude mice. These data suggest that the anti-DR5 chimeric antibody HMCAZ5 may have a clinical use and represents a useful immunological strategy, in combination with chemotherapy, for the treatment of cancer ? 2012 IUBMB Life, 64(9): 757-765, 2012.     

组织工程的新来源--原始生殖细胞

原始生殖细胞具备发育全能性,因数量较多,所以进行分离克隆将优于数目较少的内细胞团细胞。可作为组织工程的新来源：原始生殖细胞是研究基因组印迹与胚胎早期发育关系的最佳材料,还是研究生殖细胞发育分化的体外模型和研究转基因动物遗传操作的有效载体．具有广泛的应用前景。     

一种单个胚胎的DNA模板制备方法

建立了一种简单处理单个卵子和早期胚胎制备DNA模板的方法——KOH/DTT-Triton X裂解法,并与TE-蛋白酶K法比较了PCR扩增效率。结果,采用KOH/DTT-Triton X裂解法处理单个卵子或2-细胞胚、8-细胞胚、桑椹胚、囊胚后,作为DNA模板直接进行PCR扩增线粒体DNA片段,3对引物的PCR扩增总成功率为100%（70/70）,而TE-蛋白酶K法处理的单个卵子的PCR扩增总成功率为92.9%（65/70）,二者差异显著（P<0.05）。但两种方法所制备模板的PCR假阳性率均为0。实验设计的KOH/DTT-Triton X裂解法是一种有效的单个早期胚胎的DNA模板制备方法,经一次PCR扩增即能获得清晰的目的DNA条带,能够满足早期胚胎遗传物质检测的需要。