林下层植物在退化马尾松林恢复初期养分循环中的作用

以鼎湖山退化马尾松 (Pinusmassoniana)林恢复过程中林下层植物凋落物、分解和养分动态为对象 ,研究了林下层植物在退化马尾松林恢复初期养分循环中的作用。结果表明 ,林下层年凋落物量除在第 5年有所下降外均随时间逐年上升 ,但其增加速率随年份不同而异 ,总平均年增长速率为 3 8%。第 4年凋落物量为 0 .2 0 t· hm- 2 · a- 1,第 1 1年为 1 .1 7t·hm- 2·a- 1。凋落物养分元素平均浓度为 (% ) :N0 .95 ,P0 .0 4,K0 .5 7,Ca0 .1 3和 Mg0 .0 8,基本上以夏季和秋季最高冬春交替月份最低。第 1 1年凋落物各元素养分归还量为 (kg· hm- 2·a- 1) :N1 1 .1 0 ,P0 .47,K6.65 ,Ca1 .48和 Mg 0 .91。凋落物在分解过程中失重率呈直线模型变化 ,第 1年的分解速率为 3 1 % ,至试验结束时凋落物的残存量占起始量的 66%。在凋落物分解过程中 ,N和 P浓度随时间逐渐上升 ,但 N增加的速度较 P快 ,其余元素浓度均下降 ,但 K下降的速度最快。在凋落物分解过程中 ,N是唯一表现残留量呈先上升然后下降变化的元素。P的残留量变化与凋落物的失重率变化几乎一致。各元素在分解试验结束时残留量占起始量的百分比分别为 :N 90 % ,P 67% ,K 9% ,Ca 3 0 %和Mg 1 4%。可见 ,林下层凋落物在退化马尾松林恢复初期碳及其它营养元素循     

一个母系遗传非综合征耳聋大家系mtDNA序列分析

通过分析本家系mtDNA序列,探讨淮阴一非综合征耳聋大家系患病的分子遗传学机制.采用聚合酶链反应(PCR)扩增mtDNA与非综合征耳聋相关位点nt1555、nt7445的区域和人类种群研究的D-loop区、PCR-异源双链分析、PCR-RFLP、PCR产物克隆序列测定等技术对该家系进行了系统的研究.发现该家系中全部母系亲属有mtDNAA1555G突变,而家系中非母系个体、对照组(100例正常个体)的mtDNA1555位点均为A.该家系mtDNA7445位点无突变;该家系属于II型线粒体;发现家系D-loop区存在未见报道的碱基插入.提示mtDNAA1555G位点突变可能是导致该家系患者致聋的主要因素之一.遗传背景可能对家系疾病的表型存在一定程度的影响。 Abstract:We find an extensive nonsyndromic sensorineural deafness family in Huaiyin,and investigate the possible molecular genetic mechanism of matrilineal nonsyndromic sensorineural deafness.We use PCR,combined with PCR-heteroduplex analysis,PCR-RFLP and sequencing techniques to examine part of 12S rRNA,tRNAser(UCN),and D-loop region of this pedigree.1)We found an A to G transition at position 1555(A1555G) of the mitochondrial 12S rRNA from all the patients and four matrilineal.2)An new nucleotide insertion was indentified in D-Loop region.3)According to the polymorphism of D-loop,this pedigree belong to mitochondrial type II.The study showed that the A1555G mutation may be one of major factors in progressive inherited deafness of this family and genetic background should be investigated in the future.     

赤子爱胜蚓（Eisenia foetida）中抗肿瘤与纤溶酶原激酶活性蛋白质的分离与鉴定

采用SephadexG 75和HiPrep 1 6 / 6 0DEAE离子交换等方法从赤子爱胜蚓 (Eiseniafoetida)中提取到一组活性蛋白质成分 ,双向电泳分析证明它们为一组pI在 3 .0～ 4 .0之间的酸性蛋白质 ;利用体外K5 6 2、HeLa、SY5Y等肿瘤细胞抑制实验和纤维蛋白平板实验 ,跟踪测定活性 ,证明乙醇沉淀组分D2 (8)是既具肿瘤抑制 ,又具有激酶活性的蛋白质成分。同时应用非变性电泳对乙醇沉淀组分进行分离 ,并利用电洗脱、凝胶原位酶解和ESI MS等蛋白质组学方法 ,鉴定了其中 6种蛋白质的分子量、氨基酸组成、N末端序列和肽质量指纹图信息 ,其中条带 9与D2 (8)组分为同一种蛋白质 ;研究证明蚯蚓中含有既具抗肿瘤活性又具有激酶活性的蛋白质成分。采用的方法可适用于活性蛋白质成分的整体分离与鉴定     

Les génotypes responsables de mucoviscidose ou d’absence bilatérale des canaux déférents ABCD

Over the last decade, the genetic basis for CBAVD has been identified by its association with CFTR gene mutations, and CBAVD is now generally considered to be a mild or incomplete form of CF. In this review, the author summarizes the main results of compilation of CFTR gene analysis conducted in French laboratories for 3,923 patients with CF and 800 males with CABVD. The degree of clinical expression can be affected by several variables, including the molecular mechanisms by which the various CFTR mutations impair or disrupt the function of the CFTR chloride channel. Phenotypic expression of CFTR mutational genotypes varies from severe, progressive pulmonary disease with pancreatic insufficiency (CF-PI), to mild pulmonary disease with pancreatic sufficiency (PS) or singleorgan forms of “CFTR-opathies”. In CF, a total of 310 different CFTR mutations accounting for 94% of 7,846 CF alleles have generated almost 500 different genotypes, comprising 2 severe mutations in 88% of cases (CF-PI), one severe mutation in trans to a mild mutation in 11% (CF-PS), and 2 mild mutations in 1% of identified genotypes. In CBAVD, 137 mutations scattered over the whole gene were identified in 60% of 1,600 CBAVD alleles during the study. Among the 150 characterized mutational CFTR genotypes, compound heterozygosity was the rule, and the most frequent CBAVD combinations were ΔF508/5T (35%), ΔF508/other mutation (30%, including ΔF508/R117H-7T: 5,6%), and 5T/other mutation (17%). No combination of two severe mutations was found in CBAVD (0%); by contrast with the CF population, 88% of genotypes identified in CBAVD comprised a severe mutation in trans to a mild mutation, and 12% consisted of 2 mild mutations. A total of 22 genotypes were shared by both CF and CBAVD. The role of the 5T allele as a splicing variant with variable, incomplete disease penetrance in CBAVD is reviewed. Other haplotype backgrounds, such as the TG12 sequence and the M470V polymorphism, may influence CFTR splicing and/or function. This study confirms the high molecular heterogeneity of CFTR mutations in CBAVD and emphasizes the importance of extensive CFTR analysis in these patients. Longterm follow-up studies of CBAVD patients are necessary in order to predict the phenotypic consequences of numerous CFTR mutational genotypes.     

人骨形成蛋白-2C端102肽的诱骨活性

为分析更短的Hbmp-2C端肽是否具有诱骨活性 ,寻求新型的有诱骨活性的基因工程Hbmp-2产品。利用温度诱导的大肠杆菌表达系统表达肽段长度为102个氨基酸的Hbmp-2C端肽及其Cys的突变体。表达产物经纯化复性后 ,植入小鼠肌袋模型中测试其诱骨活性。获得了能稳定表达Hbmp 2C端肽的工程菌 ,测序结果与预期的序列完全一致。表达产物以包涵体形式存在 ,表达量占细胞总蛋白的 3 0 %。产物经纯化复性后 ,小鼠肌袋模型测试结果表明 :Hbmp 2 10 2肽仍具有诱骨活性 ,而将C端第一位Cys突变的 10 2肽诱骨活性丧失。实验表明 :比Hbmp 2成熟肽 ( 114个氨基酸 )更短的C端 10 2肽仍具有良好诱骨活性 ,这 10 2肽N端第一个Cys对其诱骨活性可能是必需的。     

雷公藤鲨烯环氧酶基因克隆与表达分析

以雷公藤(Tripterygium wilfordii Hook.f.)发状根为试验材料,采用RT-PCR方法,克隆得到2个雷公藤鲨烯环氧酶编码基因,命名为TwSE1(GenBank登录号MG717395)和TwSE2(GenBank登录号MG717396)。序列分析表明,TwSE1和TwSE2的开放阅读框分别为1 578和1 584bp,分别编码525和527个氨基酸,2条序列相似性为76.18%,但N端序列不保守。实时荧光定量PCR检测雷公藤鲨烯环氧酶在不同组织部位的表达模式,以及雷公藤发状根受茉莉酸甲酯(MeJA)诱导后基因表达的结果表明,TwSE1、TwSE2基因在雷公藤根、茎、嫩叶、老叶、花中均有表达,TwSE1在花中表达丰度最高,在根中表达丰度最低;但TwSE2在花和嫩叶中表达量最高,在老叶中表达量最低,且TwSE2在各组织部位的表达量都低于TwSE1。雷公藤发状根经MeJA诱导后,TwSE1、TwSE2基因表达量均上升,都表现为表达量先上升后下降再上升的趋势,并于诱导后3h达到一个高水平表达,之后下降,在诱导12h后表达量又迅速上升;在相同诱导条件下,TwSE2基因表达水平的提高小于TwSE1基因。     

水牛卵巢黄体形成和退化的蛋白质表达谱构建及生物信息学分析

本研究构建了水牛卵巢黄体形成及退化过程的定量蛋白质表达谱,从中寻找与水牛发情周期相关的重要蛋白质。为研究水牛卵巢周期性变化的分子机制提供蛋白质水平的数据支撑,进而为提高水牛繁殖效率奠定实验基础。以水牛排卵后的红体期(corpus hemorrhagicum,CH)、黄体期(corpus luteum,CL)和白体期(corpus fibrosum,CF)的卵巢作为研究对象,利用串联质谱标签(tandem mass tag,TMT)标记结合液质联用((liquid chromatography/mass spectrometry,LC-MS/MS)的定量蛋白质组学技术,采用相关软件对得到的差异表达蛋白质进行生物信息学分析。同时对与水牛发情周期相关的重要差异蛋白质:单核巨噬细胞分化抗原(CD14)、通用转录因子Ⅱ-Ⅰ(GTF2I)、羟基类固醇(17β)脱氢酶1(HSD17B1)、U6 sn RNA相关Sm样蛋白质(LSM1)和纤溶酶原激活物抑制物(SERPINE1)进行了qRT-PCR分析验证。结果显示,共鉴定得到2 343种蛋白质,其中差异表达蛋白质有284种(差异倍数≥2.0),初步构建了水牛卵巢黄体形成和退化的定量蛋白质表达谱。对其中的五种重要差异蛋白质(CD14、GTF2I、HSD17B1、LSM1和SERPINE1)进行qRT-PCR验证,结果有四种(CD14、HSD17B1、LSM1和SERPINE1)的qPCR结果与质谱结果相一致,仅GTF2I与质谱结果不一致,可能是由于GTF2I存在转录后调控。本研究首次从蛋白质水平对水牛卵巢排卵后的周期性变化的分子机制进行了探究,同时为其他家畜品种发情周期的研究提供了新的研究思路。     

<Emphasis Type="Italic">NmEXT</Emphasis> Extensin Gene: a Positive Regulator of Resistance Response Against the Oomycete <Emphasis Type="Italic">Phytophthora nicotianae</Emphasis>

The oomycete pathogens produce important diseases in many plant species. To identify extensin genes expressed during the oomycete Phytophthora nicotianae-Nicotiana megalosiphon interaction, we used the SuperSAGE technology. Using this approach, we detected a N. megalosiphon extensin gene (NmEXT) triggered during the interaction. The extensin gene accumulation induced by the pathogen correlated with disease resistance in different Nicotiana species. Transient expression of NmEXT gene in susceptible Nicotiana tabacum enhanced the resistance to P. nicotianae. Our date indicated that NmEXT gene served a positive role in N. tabacum resistance against P. nicotianae.