二元融合子与荧光假单胞菌耐药性遗传标记的筛选

应用定性和定量药物敏感性试验与诱变相结合,筛选出荧光假单胞菌56-12-10菌株的遗传标记为链霉素抗性,二元融合子AM-1菌株的遗传标记为环丙沙星抗性,确定了在这两种细菌原生质体融合试验中,选择培养基中链霉素的应用浓度为300Iu/ml,环丙沙星应用浓度为100Iu/ml。     

RT—PCR法检测大鼠脑组织及C6细胞中β—APP的表达

β-淀粉样蛋白(β-AP)是阿尔茨海默氏病(Alzheimer’s disease)病人老年斑的主要成分,它是β-淀粉样前体蛋白(β-APP)剪切后的产物。β-APP基因在体内存在β-APP_(695),β-APP_(751)β-APP_(770)。等几种主要的转录物,它们的区别在于Kunize丝氨酸蛋白酶抑制区(KDI)编码序列的存在和缺失。通过RT-PCR技术,用针对KPI编码区两侧序列的一种特异性引物可由总RNA样品中扩增出反映以上三种转录物的cDNA片段。实验表明,胎鼠脑组织中未检测到β-APPmRNA;6月龄大鼠海马组织,大脑皮层中只检测到β-APP_(695);在神经胶质瘤细胞系C6中存在β-APP_(695),β-APP_(751),β-APP_(770),其中β-APP_(770)占优势。     

Nuclear targeting signal recognition: a key control point in nuclear transport?

Recent progress indicates that there are multiple pathways of nucleocytoplasmic transport which involve specific targeting sequences, such as nuclear localization sequences (NLSs), and cytosolic receptor molecules of the importin/karyopherin superfamily which recognise and dock the NLS-containing proteins at the nuclear pore. This first step of nuclear import/export is of central importance, with the affinity of the importin-targeting sequence interaction a critical parameter in determining transport efficiency. Different importins possess distinct NLS-binding specificities, which allows the system to be modulated through differential expression of the importins themselves, as well as through competition between different importins for the same protein, and between different proteins for the same importin. The targeting sequence-importin interaction can also be influenced directly by phosphorylation increasing the affinity of the interaction with importins or by targeting sequence masking through phosphorylation or specific protein binding. Targeting sequence recognition thus appears to represent a key control point in the regulation of nuclear transport. BioEssays 22:532-544, 2000.     

Blockade of L-type voltage-gated Ca channel inhibits ischemia-induced neurogenesis by down-regulating iNOS expression in adult mouse

Neurogenesis in the adult mammalian hippocampus may contribute to repairing the brain after injury. The signals that regulate neurogenesis in the dentate gyrus following ischemic stroke insult are not well known. We have previously reported that inducible nitric oxide synthase (iNOS) expression is necessary for ischemia-stimulated neurogenesis in the adult dentate gyrus. Here, we show that mice subjected to 90 min of middle cerebral artery occlusion (MCAO) significantly increased the number of new neurons and up-regulated iNOS expression in the dentate gyrus. Blockade of the L-type voltage-gated Ca(2+) channel (L-VGCC) prevented neurogenesis in the dentate gyrus and subventricular zone (SVZ), and down-regulated iNOS expression in the dentate gyrus after cerebral ischemia. This study suggests that Ca(2+) influx through L-VGCC is involved in ischemia-induced neurogenesis by up-regulating iNOS expression.     

Kinetic FP-TDI assay for SNP allele frequency determination

Strategies for identifying genetic risk factors in complex diseases by association studies require the comparison of allele frequencies of numerous SNPs between affected and control populations. Theoretically, hundreds of thousands of SNP markers across the genome will have to be genotyped in these studies. Genotyping SNPs one sample at a time is extremely costly and time consuming. To streamline whole genome association studies, some have proposed to screen SNPs by pooling the DNA samples initially for allele frequency determination and perform individual genotyping only when there is a significant discrepancy in allele frequencies between the affected and control populations. Here we describe a new method for determining the allele frequency of SNPs in pooled DNA samples using a two-color primer extension assay with real-time monitoring of fluorescence polarization (named kinetic FP-TDI assay). By comparing the ratio of the rate of incorporation of the two allele-specific dye-terminators, one can calculate the relative amounts of each allele in the pooled sample. The accuracy of allele frequency determination with pooled samples is within 3.3 +/- 0.8% of that determined by genotyping individual samples that make up the pool.     

寄生革翅目蠼螋的被毛孢一新种

在湖北省神农架林区采集到一种寄生于蠼螋成虫的真菌标本snj121022,分离并获得菌株 GZUIFR-snj121022,经形态学、系统发育和拆分网络综合分析,鉴定其为被毛孢属的一个新种,命名为神农架被毛孢Hirsutella shennongjiaensis。本文对其进行了详细的形态特征描述、图解和系统发育分析。     

Amplification activation loop between caspase-8 and -9 dominates artemisinin-induced apoptosis of ASTC-a-1 cells

Although caspases have been demonstrated to be involved in artemisinin (ARTE)-induced apoptosis, their exact functions are not well understood. The aim of this report is to explore the roles of caspase-8, -9 and -3 during ARTE-induced apoptosis in human lung adenocarcinoma (ASTC-a-1) cells. ARTE treatment induces a rapid generation of reactive oxygen species (ROS), and ROS-dependent apoptosis as well as the activation of caspase-8, -9 and -3 via time- and dose-dependent fashion. Of upmost importance, inhibition of caspase-8 or -9, but not caspase-3, almost completely blocks the ARTE-induced not only activation of the caspase-8, -9 and -3 but also apoptosis. In addition, the apoptotic process triggered by ARTE does not involve the Bid cleavage, tBid translocation, significant loss of mitochondrial membrane potential and cytochrome c release from mitochondria. Moreover, silencing Bax/Bak does not prevent the ATRE-induced cell death as well as the activation of caspase-8, -9 and -3. Collectively, our data firstly demonstrate that ARTE triggers a ROS-mediated positive feedback amplification activation loop between caspase-8 and -9 independent of mitochondria, which dominantly mediated the ARTE-induced apoptosis via a caspase-3-independent apoptotic pathway in ASTC-a-1 cells. Our findings imply a potential to develop new derivatives from artemisinin to effectively initiate the amplification activation loop of caspases.     

昆虫保幼激素促进家蚕杆状病毒系统的基因表达

杆状病毒表达载体系统(Baculovirus Expression VecterSvstem,BEVS)的一个最大优点是外源基因的高效表达(Hy-perexpression).但是,不同的外源基因在BEVS系统中的表达水平相差很大,较低的如α-干扰素,表达量为1～5mg/L培养细胞;高的如β-半乳糖苷酶,表达量可达600mg/L培养细胞.外源基因在BEVS系统中表达量受到诸多因素的影响,如细胞的类型与质量,外源基因蛋白的性质,启动子序列的完整性,是否为融合蛋白等[1].如何使外源基因在BEVS系统中高效表达,是近年来该领域中研究最活跃的方向之一.已证实家蚕杆状病毒的表达量受宿主遗传型的影响,最低和最高的遗传型相差达7倍以上[2].林水中等发现家蚕饲料中添食适当浓度的硫酸铜可提高外源基因单位表达量10%左右[3].杆状病毒在复制循环中表现出两种类型:芽生病毒和包涵体病毒,其中芽生病毒引起宿主体内不同组织间的感染,包涵体病毒则引起宿主之间感染[1].杆状病毒基因组中蜕皮激素尿苷二磷酸葡萄糖基转移酶(egt)基因影响激素在宿主体内的平衡[4],egt基因通过糖基化作用使蜕皮激素失活,打破宿主体内的激素平衡,延长幼虫期,以利于病毒的增殖[5].家蚕血淋巴中保幼激素(Juvenile hormone,JH)的滴度同样决定着幼虫发育的进程[6],本文通过体表使用保幼激素,以研究保幼激素对家蚕核型多角体病毒和宿主之间的相互关系及对外源基因表达量的影响.     

新疆罗布麻生态类型及其纤维品质研究

新疆塔里木河及叶尔羌河流域是我国能够提供商品精干罗布麻的主要地区。由于野生罗布麻生长高矮不一,形态各异,与其纤维品质的相关性较大。通过40个株号的罗布麻植株形态和纤维长度等的的测定,分析各类型罗布麻的纤维长度和罗布麻植株各部分纤维长度情况。研究结果表明：罗布红麻高杆类型主茎纤维最长,罗布麻放牧类型纤维最短。罗布麻植株各部分纤维长度是主茎上的大于分枝,主茎中部的最长,基部和梢部最短。为野生罗布麻资源开发利用提科学依据。