Olfactory marker protein interacts with adenosine nucleotide derivatives

Olfactory marker protein (OMP) is a genetic signature for mature olfactory receptor neurons (ORNs). Recently, it has been proposed that OMP directly captures odour-induced cAMP to swiftly terminate the olfactory signal transduction to maintain neuronal sensitivity. In the present study, we show that OMP can also interact with other adenosine nucleotides as ATP, ADP and AMP with different affinities. We performed bioluminescent resonant energy transfer (BRET) assay to measure the binding actions of the adenosine nucleotide derivatives in competition to cAMP. Amongst all, ATP showed the bell-shape affinity to OMP in the presence of cAMP; ADP and AMP showed fewer affinities to OMP than ATP. In the absence of cAMP analogues, ATP alone bound to OMP in a dose dependent manner with a lower affinity than to cAMP. Thus, OMP possessed different affinities to ATP in the presence or absence of cAMP. OMP may interact differentially with ATP and cAMP depending on its supply and demand along the cAMP-associated signalling in the limited spaces of cilia of ORNs.     

A molecular method for the detection of sally lightfoot crab larvae (Grapsus grapsus, Brachyura, Grapsidae) in plankton samples

The decapod Grapsus grapsus is commonly found on oceanic islands of the Pacific and Atlantic coasts of the Americas. In this study, a simple, quick and reliable method for detecting its larvae in plankton samples is described, which makes it ideal for large-scale studies of larval dispersal patterns in the species.     

高粱遗传转化研究进展

高粱（Sorghum bicolor）是一种重要的多用途作物, 其遗传转化研究对于高粱的分子育种和分子遗传学基础研究都具有重要意义。该文对高粱遗传转化的方法、标记基因、遗传转化的启动子和受体系统进行了综述, 并提出了今后高粱遗传转化应当集中研究的问题。     

菊苣体细胞再生植株的遗传稳定性分析

目的:研究菊苣再生植株的遗传稳定性.方法:以菊苣叶片为外植体,经第一代和第二代体细胞再生获得再生植株,分别对再生植株提取DNA,从12个引物中筛选了2个多态性好的引物,对第一代和第二代体细胞再生植株进行RAPD标记.结果:菊苣第一代体细胞无性系没有发生DNA多态性变异,第二代体细胞无性系在分子水平发生了1条DNA多态性变异.结论:RAPD分子标记方法可以鉴定菊苣组织培养过程中的遗传稳定性和遗传变异,为菊苣快繁和遗传转化奠定了基础.     

中国重要海洋动物遗传多样性的研究进展

海洋动物遗传多样性的研究不仅可以揭示物种的起源与进化历史,而且为遗传资源的保存、海水养殖动物育种和遗传改良及整个海洋生态环境的修复和稳定等工作提供理论依据.本文概述了近十几年来我国重要海洋动物(主要包括鱼类、虾蟹类和贝类)遗传多样性研究所取得的成果,具体阐述其在种质鉴定、系统进化、群体遗传结构分析和良种培育等方面的应用,以期进一步推动海洋动物遗传多样性研究,加快优良种质的培育,促进海水养殖业的健康发展,实现海洋生物资源的合理开发和可持续利用.     

中缅树鼩微卫星分子标记的筛选

目的 筛选中缅树鼩微卫星分子标记,逐步填补中缅树鼩特异性遗传标记的空白.方法 建立中缅树鼩基因小片段插入文库,利用5’端地高辛标记的(CA)15探针从约1500个菌落中选出36个阳性克隆.对这些克隆进行测序,发现其中15个含有重复序列,其中1个为重复克隆,1个因两端序列太短而不能设计引物.结果 用Primer3软件设计...     

甲状腺癌肿瘤标志物研究进展

甲状腺癌肿瘤标志物是由甲状腺癌组织和细胞产生的异常表达的生物活性物质。近年来,肿瘤标志物成为肿瘤基础和临床应用的一个非常活跃的领域,其不仅与甲状腺癌的形成、发展和转移关系密切,也对它的诊断和治疗具有重要意义。随着研究的不断深入,这些肿瘤标志物在临床上已显示出了广阔的应用前景。本文就近年来研究较多且与甲状腺癌密切相关的肿瘤标志物,包括Galectin-3,CK-19,VEGF,端粒酶和端粒酶逆转录酶,MMPs,降钙素,E-cadherin,Tg,TSHRmRNA进行综述。     

PCR-RFLP assays to distinguish the Western and Eastern phylogroups in wild and cultured tench Tinca tinca

The tench Tinca tinca is a valued table fish native to Europe and Asia, but which is now widely distributed in many temperate freshwater regions of the world as the result of human-mediated translocations. Fish are currently being transplanted between watersheds without concern for genetic similarity to wild populations or local adaptation, and efficient phylogeographic markers are therefore urgently needed to rapidly distinguish genetically distinct geographical populations and to assess their contribution to the hatchery breeds and to the stocked wild populations. Here, we present a new method to distinguish recently discovered and morphologically undistinguishable Western and Eastern phylogroups of the tench. The method relies on PCR-RFLP assays of two independent nuclear-encoded exon-primed intron-crossing (EPIC) markers and of one mitochondrial DNA (mDNA) marker and allows the rapid identification of the Western and Eastern phylogroup and also of three geographical mtDNA clades within the Eastern phylogroup. Our method will enable researchers and fishery practitioners to rapidly distinguish genetically divergent geographical populations of the tench and will be useful for monitoring the introduction and human-mediated spread of the phylogroups in wild populations, for characterization of cultured strains and in breeding experiments.     

High-throughput microsatellite isolation through 454 GS-FLX Titanium pyrosequencing of enriched DNA libraries

Microsatellites (or SSRs: simple sequence repeats) are among the most frequently used DNA markers in many areas of research. The use of microsatellite markers is limited by the difficulties involved in their de novo isolation from species for which no genomic resources are available. We describe here a high-throughput method for isolating microsatellite markers based on coupling multiplex microsatellite enrichment and next-generation sequencing on 454 GS-FLX Titanium platforms. The procedure was calibrated on a model species (Apis mellifera) and validated on 13 other species from various taxonomic groups (animals, plants and fungi), including taxa for which severe difficulties were previously encountered using traditional methods. We obtained from 11,497 to 34,483 sequences depending on the species and the number of detected microsatellite loci ranged from 199 to 5791. We thus demonstrated that this procedure can be readily and successfully applied to a large variety of taxonomic groups, at much lower cost than would have been possible with traditional protocols. This method is expected to speed up the acquisition of high-quality genetic markers for nonmodel organisms.     

Marker Density and Read Depth for Genotyping Populations Using Genotyping-by-Sequencing

Genotyping-by-sequencing (GBS) approaches provide low-cost, high-density genotype information. However, GBS has unique technical considerations, including a substantial amount of missing data and a nonuniform distribution of sequence reads. The goal of this study was to characterize technical variation using this method and to develop methods to optimize read depth to obtain desired marker coverage. To empirically assess the distribution of fragments produced using GBS, ∼8.69 Gb of GBS data were generated on the Zea mays reference inbred B73, utilizing ApeKI for genome reduction and single-end reads between 75 and 81 bp in length. We observed wide variation in sequence coverage across sites. Approximately 76% of potentially observable cut site-adjacent sequence fragments had no sequencing reads whereas a portion had substantially greater read depth than expected, up to 2369 times the expected mean. The methods described in this article facilitate determination of sequencing depth in the context of empirically defined read depth to achieve desired marker density for genetic mapping studies.