Defective Presynaptic Choline Transport Underlies Hereditary Motor Neuropathy

The neuromuscular junction (NMJ) is a specialized synapse with a complex molecular architecture that provides for reliable transmission between the nerve terminal and muscle fiber. Using linkage analysis and whole-exome sequencing of DNA samples from subjects with distal hereditary motor neuropathy type VII, we identified a mutation in SLC5A7, which encodes the presynaptic choline transporter (CHT), a critical determinant of synaptic acetylcholine synthesis and release at the NMJ. This dominantly segregating SLC5A7 mutation truncates the encoded product just beyond the final transmembrane domain, eliminating cytosolic-C-terminus sequences known to regulate surface transporter trafficking. Choline-transport assays in both transfected cells and monocytes from affected individuals revealed significant reductions in hemicholinium-3-sensitive choline uptake, a finding consistent with a dominant-negative mode of action. The discovery of CHT dysfunction underlying motor neuropathy identifies a biological basis for this group of conditions and widens the spectrum of disorders that derive from impaired NMJ transmission. Our findings compel consideration of mutations in SLC5A7 or its functional partners in relation to unexplained motor neuronopathies.     

猪CFL2b 基因cDNA克隆初步分析

利用基因表达谱芯片分析法筛选出与大白猪高肌肉产量-肌纤维形成有关的CFL2b基因.参考人和小鼠CFL2b基因序列,采用SMART-RACE技术结合EST序列拼接技术,从猪骨骼肌肌肉中首次克隆了猪CFL2b的全长cDNA序列（GenBank登录号EU561660,EU561661）,Northern杂交检测CFL2b基因 mRNA.结果表明,猪CFL2b基因含有2个转录本,长转录本3　012 bp,短转录本1　466 bp .CFL2b基因在多种真核生物中都有表达,且编码区序列非常保守,开放式读码框501 bp编码了166个氨基酸的蛋白质.氨基酸序列分析表明,猪CFL2基因与人和小鼠氨基酸同源性分别为100%和99.1%.核苷酸序列相似性分别为88.1%和74.9%.     

Anti-alpha-fodrin antibodies do not add much to the diagnosis of Sjögren's syndrome

The presence of anti-alpha-fodrin autoantibodies has been reported to be a highly specific and sensitive test for the diagnosis of Sj?gren's syndrome (SjS). We looked (in Nijmegen) for anti-alpha-fodrin, anti-Ro60, and anti-La autoantibodies in a cohort of 51 patients with rheumatic diseases (primary SjS [21], secondary SjS 6, rheumatoid arthritis [RA] 12, systemic lupus erythematosus [SLE] 6, and scleroderma 6) and in 28 healthy subjects, using ELISA, immunoblotting, and immunoprecipitation. The same samples were analyzed with an alternative anti-alpha-fodrin ELISA in Hanover. The Nijmegen ELISA of the sera from primary SjS showed sensitivities of 43% and 48% for IgA- and IgG-type anti-alpha-fodrin antibodies, respectively. The Hanover ELISA showed sensitivities of 38% and 10% for IgA- and IgG-type anti-alpha-fodrin antibodies, respectively. The ELISAs for alpha-fodrin showed six (Nijmegen) and four (Hanover) anti-alpha-fodrin-positive RA sera. IgA and IgG anti-fodrin antibodies were also present in four patients with secondary SjS. The sensitivities of Ro60 and La-antibodies in the Nijmegen ELISA were 67% and 62%, respectively. Unlike anti-alpha-fodrin antibodies, all anti-Ro60 and anti-La positive sera could be confirmed by immunoblotting or RNA immunoprecipitation. Thus, anti-Ro and anti-La autoantibodies were more sensitive than anti-alpha-fodrin autoantibodies in ELISA and were more frequently confirmed by other techniques. Anti-La antibodies appear to be more disease-specific than anti-alpha-fodrin antibodies, which are also found in RA sera. Therefore, the measurement of anti-alpha-fodrin autoantibodies does not add much to the diagnosis of Sj?gren's syndrome.     

Melon rugose mosaic virus, the cause of a disease of watermelon and sweet melon

A mechanically transmissible virus with isometric particles c. 32 nm in diameter, was isolated from infected watermelons and sweet melons in the People's Democratic Republic of Yemen. Purified virus preparations contained two major sedimenting components with sedimentation coefficients of 61S and 117S. In isopycn ic centrifugation in CsCl the particles formed a single band of buoyant density 1.39 g cm^-3. Preparations of virus particles comprised of a single polypeptide of mol. wt c. 22 000 and ssRNA of mol. wt 2.1 × 10⁶. The virus was serologically related to three of six subgroups of tymoviruses tested. The name melon rugose mosaic virus is proposed for this newly described virus.     

文蛤的生物沉积和呼吸排泄过程及其在双台子河口水层-底栖系统中的耦合作用

为揭示河口埋栖性双壳贝类优势种类在水层——底栖系统中的生态耦合作用,利用生物沉积物捕集器和封闭式代谢瓶,于双台子河口现场研究了文蛤主要生理生态过程如生物沉积速率、耗氧率、排氨率和排磷率的季节变化。结果表明,文蛤的生物沉积速率、耗氧率、排氨率及排磷率均具有明显的季节变化:夏季最高,冬季最低。二龄及三龄文蛤个体的生物沉积速率周年变化分别为0.02—0.30 g-1个-1d-1、0.06—0.60 g-1个-1d-1;耗氧率变化分别为0.45—16.64 mg-1个-1d-1、1.03—30.51 mg-1个-1d-1;排氨率季节变化分别为0.001—0.14 mg-1个-1d-1、0.002—0.28 mg-1个-1d-1;排磷率季节变化分别为0.002—0.069 mg-1个-1d-1、0.003—0.16 mg-1个-1d-1。文蛤的生物沉积速率及呼吸排泄速率均受龄期制约:在同一季节,文蛤的单位个体生物沉积速率及呼吸和排泄速率均表现为二龄三龄。方差分析显示,季节、龄期及两者交互作用对文蛤生物沉积速率、耗氧率、排氨率及排磷率均有显著影响。基于不同季节双台子河口文蛤生物量(0.67个/m2、2.4 g/m2),估算出文蛤种群每年向该河口排放大约5321.90 t生物沉积物(干重)、1.43 t NH+4-N和0.93 t PO3-4-P,并且消耗大约221.59 t O2。研究结果表明,文蛤通过生物沉积及呼吸排泄作用,大大加强了双台子河口沉积物-水界面的物质交换通量,在双台子河口水层-底栖系统耦合作用中扮演着重要生态角色。     

扎龙湿地硅藻植物群落季节变化及其对环境的响应

扎龙湿地位于黑龙江省西部、松嫩平原乌裕尔河下游,是我国北方同纬度地区最完整的湿地。于2012年春、夏、秋3季,对扎龙湿地6个代表性区域进行硅藻标本采集,经观察鉴定,发现硅藻植物140个分类单位,包括121种19变种,隶属于2纲6目9科30属。羽纹纲物种较丰富,占总种类数的95%。硅藻植物群落呈现明显的季节演替,秋季硅藻种类丰富度及相对丰度明显高于春、夏两季,优势种多以淡水、半咸水、喜弱碱的种类为主,优势种与水体的盐度和酸碱度存在一定的响应关系。应用典范对应分析(Canonical Correspondence Analysis,CCA)探讨硅藻植物群落变化与环境因子之间的关系。CCA结果显示在扎龙湿地中,水温、电导率、pH、溶解氧是影响硅藻群落结构变化的主要因素,此外总氮、总磷也是硅藻群落季节演替的重要驱动因子。结合硅藻植物多样性指数和硅藻商对扎龙湿地水质进行综合评价,结果显示扎龙湿地整体为中-寡污带水体,部分水域水质较清洁,少数样点受人为因素影响,呈轻污染。     

Detection of two loci involved in (1-->3)-beta-glucan (curdlan) biosynthesis by Agrobacterium sp. ATCC31749, and comparative sequence analysis of the putative curdlan synthase gene

Genes essential for the production of a linear, bacterial (1-->3)-beta- glucan, curdlan, have been cloned for the first time from Agrobacterium sp. ATCC31749. The genes occurred in two, nonoverlapping, genomic fragments that complemented different sets of curdlan( crd )-deficient transposon-insertion mutations. These were detected as colonies that failed to stain with aniline blue, a (1-->3)-beta-glucan specific dye. One fragment carried a biosynthetic gene cluster (locus I) containing the putative curdlan synthase gene, crdS, and at least two other crd genes. The second fragment may contain only a single crd gene (locus II). Determination of the DNA sequence adjacent to several locus I mutations revealed homology to known sequences only in the cases of crdS mutations. Complete sequencing of the 1623 bp crdS gene revealed highest similarities between the predicted CrdS protein (540 amino acids) and glycosyl transferases with repetitive action patterns. These include bacterial cellulose synthases (and their homologs), which form (1-->4)-beta-glucans. No similarity was detected with putative (1-->3)- beta-glucan synthases from yeasts and filamentous fungi. Whatever the determinants of the linkage specificity of these beta-glucan synthases might be, these results raise the possibility that (1-->3)-beta-glucans and (1-->4)-beta-glucans are formed by related catalytic polypeptides.      

汉滩病毒M、S基因不同拼接方式在昆虫细胞中融合表达效果比较

将汉滩病毒囊膜糖蛋白G1与核蛋白(NP)部分片段以不同方式拼 接,构建G1S0.7或S0.7G1嵌合基因,分别插入杆状病毒表达载体pFBD,转化DH10Bac致敏菌, 获得含有嵌合基因的重组穿梭质粒Bacmid,用其转染Sf9细胞,快速筛选出含有G1S0.7或S0.7 G1嵌合 基因的重组杆状病毒,在昆虫细胞中表达外源融合蛋白.利用间接免疫荧光、ELISA和免疫 印迹对表达产物进行检测.结果表明,含G1S0.7嵌合基因之重组杆状病毒可在昆虫细胞中表 达出融合蛋白,该蛋白可被抗汉滩病毒核蛋白及糖蛋白G1特异性单抗所识别,其分子量约97 kD;含S0.7G1嵌合基因之重组杆状病毒在昆虫细胞中表达的融合蛋白,只能被抗汉滩病毒核 蛋白特异性单抗所识别,其分子量约43kD.上述结果提示,G1S0.7嵌合基因可能在昆虫细胞 中表达出完整的具有生物学活性的融合蛋白,S0.7G1嵌和基因的昆虫细胞表达产物不完整 ,且生物学活性不如G1S0.7嵌合基因的表达产物.