五种豆科种子胚乳细胞的微观结构的比较

运用光学显微镜和电子显微镜分别对胡芦巴、野皂荚、皂荚、瓜尔豆、塔拉豆等五种豆科种子内胚乳细胞的形态、大小、壁厚等微观结构进行了观察比较。研究结果表明：五种种子内胚乳细胞壁几乎完全由胶状的透明的半乳甘露聚糖所填充,细胞的形态、大小差异较大,瓜尔豆、塔拉豆的内胚乳细胞呈球形或近球形;胡芦巴内胚乳细胞为多角形或多角椭圆形,它们细胞壁界限清晰,细胞排列整齐有规律;皂荚、野皂荚则为不规则的长椭球形,细胞壁彼此连接成片,界限模糊。一般地说：当细胞壁壁厚小于4μm时,胚乳胶粉中的水不溶物含量较低,1％浓度的胶液的粘度较高,而当壁厚大于4μm时,情况反之。本文的研究目的是为植物胶生产、加工提供一定的细胞学方面的依据。     

鼻腔接种伤寒杆菌Fe-SOD对鼠伤寒杆菌攻击小鼠的免疫保护作用

为探讨鼻腔接种伤寒杆菌Fe-SOD对鼠伤寒杆菌攻击小鼠的交叉免疫保护作用,用IL－1作为佐剂,将伤寒杆菌Fe-SOD经鼻腔接种小鼠,再以不同剂鼠伤寒杆菌攻击,观察小鼠的存活情况,当用IL－1作为佐剂时,经鼻腔接种伤寒杆菌Fe-SOD的小鼠在2LD50鼠伤寒杆菌攻击后,3天和7天的存活率均明显高于对照组（P＜0．01或P＜0．05）,当以5LD50鼠直菌攻击时,小鼠7天的存活率明显高于对照组（P＜0．01）。结果说明伤寒杆菌Fe-SOD经鼻腔接种后对鼠伤寒杆菌的攻击可产生一定的免疫保护作用,也进一步说明了Fe-SOD是沙门氏菌的共同保护性抗原。     

I型单纯疱疹病毒胸苷激酶真核表达载体的构建及其表达鉴定

为构建单纯疱疹病毒I型胸苷激酶(HSV1TK)的真核表达载体pcDNA3.1-EGFP/HSV1TK,鉴定其在真核细胞中的表达和功能.以pORF-HSV1TK为模板,PCR扩增的目的基因HSV1TK片段与pMD18-T载体相连接构建重组克隆pMD18-T/HSV1TK.再双酶切出HSV1TK片段,插入pcDNA3.1-EGFP多克隆位点,构建pcDNA3.1-EGFP/ HSV1TK真核表达载体并进行酶切、测序鉴定[1].分别用荧光显微镜观察和RT-PCR方法检测脂质体介导pcDNA3.1-EGFP/ HSV1TK在卵巢癌细胞SKOV3的表达;分别用MTT法和光镜检测胸苷激酶/丙氧鸟苷(HSV1TK/GCV)系统对SKOV3体外杀伤作用及旁观者效应.结果表明,重组载体酶切鉴定结果与预期结果一致,基因序列与GenBank上报道的HSV1TK基因序列完全一致.荧光显微镜观察转染后的细胞发出绿色荧光;RT-PCR结果表明HSV1TK基因能在SKOV3内有效表达.MTT和光镜结果显示转染HSV1TK基因的SKOV3细胞,加入前体药物丙氧鸟苷(GCV)处理后对其有明显的杀伤作用和旁观者效应.成功构建的真核表达载体pcDNA3.1-EGFP/ HSV1TK能在SKOV3细胞中稳定表达,且HSV1TK对卵巢癌细胞株SKOV3体外有强大的杀伤作用和旁观者效应.     

植物中的水平基因转移

水平基因转移是不通过生殖而进行的遗传物质交流, 在原核生物和单细胞真核生物的进化中起着重要作用。然而, 水平基因转移在多细胞真核生物之间的发生频率以及对多细胞真核生物进化的影响尚不明确。近期的一些研究显示, 水平基因转移在高等植物之间以及高等植物和其它生物之间普遍存在。该文将对高等植物中已发现的一些水平基因转移现象进行综述, 并尝试解析植物之间水平基因转移可能的机制及其重要意义。     

Fed-batch cultivation ofEscherichia coli YK537 (pAET-8) for production ofphoA promoter-controlled human epidermal growth factor

Secretion of the expressed heterologous proteins can reduce the stress to the host cells and is beneficial to their recovery and purification. In this study, fed-batch cultures ofEscherichia coliYK537 (pAET-8) were conducted in a 5-L fermentor for the secretory production of human epidermal growth factor (hEGF) whose expression, was under the control of alkaline phosphatase promoter. The effects of feeding of glucose and complex nitrogen sources on hEGF production were investigated. When the fed-batch culture was conducted in a chemically defined medium, the cell density was 9.68 g/L and the secreted hEGF was 44.7 mg/L in a period of 60 h. When a complex medium was used and glucose was added in pH-stat mode, the secreted hEGF was improved to 345 mg/L. When the culture was fed with glucose at a constant specific rate of 0.25 gg⁻¹h⁻¹, hEGF reached 514 mg/L. The effects of adding a solution containing yeast extract and tryptone were further studied. Different rate of the nitrogen source feeding resulted in different levels of phosphate and acetic acid formation, thus affected hEGF expression. At the optimal feeding rate, hEGF production achieved 686 mg/L.     

血痕Chelex 100抽提DNA用于人类TNF-α基因启动子区SNP分型

建立快速、简便的血样本采集及DNA抽提方法,可用于大规模的分子流行病学调查及群体遗传学研究。采用无菌纱布为载体取血,Chelex100快速抽提DNA,用TaqMan MGB探针对人类TNF-α基因启动子区-857（C／T）位点进行SNP分型。344份血样均得到明确的分型结果,获得的荧光信号强,本底低。深圳地区汉族群体-857位点基因型频率分别为：cc为0.78,ct为0.21,tt为0.01。血痕Chelex100抽提DNA为大规模血样本的采集,DNA的抽提提供了有效的手段。     

FABP4基因在阿勒泰羊尾脂沉积与代谢模型中的表达变化规律

FABP4(Fatty acid binding protein 4)参与细胞内脂肪酸的转运和脂肪酸代谢,是当前研究动物脂肪沉积与代谢的热门候选基因。为了研究FABP4基因在绵羊尾脂沉积与代谢中的作用,文章采用生物信息学方法分析了FABP4氨基酸序列在各物种中的保守性;利用半定量RT-PCR方法检测了该基因在阿勒泰羊主要组织中的表达;采用饥饿法成功建立了模拟阿勒泰羊尾脂沉积与代谢的动物模型,利用qPCR和iTRAQ(isobaric tags for relative and absolute quantitation)技术同时验证FABP4基因mRNA和蛋白在阿勒泰羊非饥饿组与饥饿组尾脂中的表达变化。序列分析结果表明,绵羊FABP4氨基酸序列在物种间高度保守,提示FABP4基因可能由于其重要的生物功能而在进化中表现出其物种的保守性。组织表达谱结果显示,FABP4 mRNA在阿勒泰羊肠脂与尾脂中均高丰度表达,暗示FABP4基因可能在脂肪中行驶着重要的生理生化功能。qPCR与iTRAQ结果显示,FABP4 mRNA与蛋白在两种极端条件下尾脂中的表达差异均不显著(P>0.05),表明FABP4基因可能不是绵羊尾脂沉积与代谢两种极端差异表型的决定基因。以上研究结果为进一步研究FABP4基因在绵羊尾脂中的生物功能奠定了基础。     

DDX39 as a predictor of clinical prognosis and immune checkpoint therapy efficacy in patients with clear cell renal cell carcinoma

DEAD-box protein 39 (DDX39) has been demonstrated to be a tumorigenic gene in multiple tumor types, but its role in the progression and immune microenvironment of clear cell renal cell cancer (ccRCC) remains unclear. The aim of the present study was to investigate the role of DDX39 in the ccRCC tumor progression, immune microenvironment and efficacy of immune checkpoint therapy.The DDX39 expression level was first detected in tumors in the public data and then verified in ccRCC samples from Changzheng Hospital. The prognostic value of DDX39 expression was assessed in the Cancer Genome Atlas (TCGA) and ccRCC patients from Changhai Hospital. The role of DDX39 in promoting ccRCC was analyzed by bioinformatic analysis and in vitro experiments. The association between DDX39 expression and immune cell infiltration and immune inhibitory markers was analyzed, and its value in predicting the immune checkpoint therapy efficacy in ccRCC were evaluated in the public database. DDX39 expression was elevated in Oncomine, GEO and TCGA ccRCC databases, as well as in Changzheng ccRCC samples. In TCGA ccRCC patients, increased DDX39 expression predicted worse overall survival (OS) (p<0.0001) and progression-free interval (PFI) (p<0.0001), and was shown as an independent predictive factor for OS (p=0.002). These findings were consistent with those from Changhai ccRCC patients. In addition, GO and GSEA analysis identified DDX39 as a pro-ccRCC gene. In vitro experiments confirmed the role of DDX39 in promoting ccRCC cell. Finally, DDX39 was found to be positively correlated with a variety of immune inhibitory markers, and could predict the adverse efficacy of immune checkpoint therapy in TIDE analysis. In conclusion, Increased DDX39 in ccRCC patients predicted worse clinical prognosis, promoted ccRCC cell proliferation, migration and invasion, and also predicted adverse efficacy of immune checkpoint therapy.