989 resultados para Marcadores de DNA
Resumo:
The mucus surface layer of corals plays a number of integral roles in their overall health and fitness. This mucopolysaccharide coating serves as vehicle to capture food, a protective barrier against physical invasions and trauma, and serves as a medium to host a community of microorganisms distinct from the surrounding seawater. In healthy corals the associated microbial communities are known to provide antibiotics that contribute to the coral’s innate immunity and function metabolic activities such as biogeochemical cycling. Culture-dependent (Ducklow and Mitchell, 1979; Ritchie, 2006) and culture-independent methods (Rohwer, et al., 2001; Rohwer et al., 2002; Sekar et al., 2006; Hansson et al., 2009; Kellogg et al., 2009) have shown that coral mucus-associated microbial communities can change with changes in the environment and health condition of the coral. These changes may suggest that changes in the microbial associates not only reflect health status but also may assist corals in acclimating to changing environmental conditions. With the increasing availability of molecular biology tools, culture-independent methods are being used more frequently for evaluating the health of the animal host. Although culture-independent methods are able to provide more in-depth insights into the constituents of the coral surface mucus layer’s microbial community, their reliability and reproducibility rely on the initial sample collection maintaining sample integrity. In general, a sample of mucus is collected from a coral colony, either by sterile syringe or swab method (Woodley, et al., 2008), and immediately placed in a cryovial. In the case of a syringe sample, the mucus is decanted into the cryovial and the sealed tube is immediately flash-frozen in a liquid nitrogen vapor shipper (a.k.a., dry shipper). Swabs with mucus are placed in a cryovial, and the end of the swab is broken off before sealing and placing the vial in the dry shipper. The samples are then sent to a laboratory for analysis. After the initial collection and preservation of the sample, the duration of the sample voyage to a recipient laboratory is often another critical part of the sampling process, as unanticipated delays may exceed the length of time a dry shipper can remain cold, or mishandling of the shipper can cause it to exhaust prematurely. In remote areas, service by international shipping companies may be non-existent, which requires the use of an alternative preservation medium. Other methods for preserving environmental samples for microbial DNA analysis include drying on various matrices (DNA cards, swabs), or placing samples in liquid preservatives (e.g., chloroform/phenol/isoamyl alcohol, TRIzol reagent, ethanol). These methodologies eliminate the need for cold storage, however, they add expense and permitting requirements for hazardous liquid components, and the retrieval of intact microbial DNA often can be inconsistent (Dawson, et al., 1998; Rissanen et al., 2010). A method to preserve coral mucus samples without cold storage or use of hazardous solvents, while maintaining microbial DNA integrity, would be an invaluable tool for coral biologists, especially those in remote areas. Saline-saturated dimethylsulfoxide-ethylenediaminetetraacetic acid (20% DMSO-0.25M EDTA, pH 8.0), or SSDE, is a solution that has been reported to be a means of storing tissue of marine invertebrates at ambient temperatures without significant loss of nucleic acid integrity (Dawson et al., 1998, Concepcion et al., 2007). While this methodology would be a facile and inexpensive way to transport coral tissue samples, it is unclear whether the coral microbiota DNA would be adversely affected by this storage medium either by degradation of the DNA, or a bias in the DNA recovered during the extraction process created by variations in extraction efficiencies among the various community members. Tests to determine the efficacy of SSDE as an ambient temperature storage medium for coral mucus samples are presented here.
Resumo:
一. 设计和筛选单链阻遏蛋白的高亲和力DNA结合序列 单链阻遏蛋白RRTRES是噬菌体434阻遏蛋白的衍生物,它是噬菌体434阻 遏蛋白的N端DBD(1-69位氨基酸)组成的共价二聚体。这个单链分子有两个DBD,一个是野生型噬菌体434的DBD-R,另一个是突变了的DBD - RTRES,二者用重组接头以头接尾的方式连接起来。在RTRES的α3-螺旋中.1、1、2、5位氨基酸与DNA识别紧密相关,它们分别为T、R、E、S。为了筛选出突变的RTRES的DNA结合位点,设计了核心序列为CATACAAGAAAGNNNNNNTTTATG随机DNA库,通过RRTRES与随机DNA库的体外结合和循环筛选。将筛选到的群体克隆并测序。通过与单链阻遏蛋白RRTRES的亲和力测定,对每一个筛选到的序列进行特性分析。结果表明,当结合位点(上述划线部分)为TTAC或TTCC时为最适操纵区序列。它们与单链阻遏蛋白RRTRES的亲和力很高,Kd值在1-10pM的范围。其中随机部分为TTTACG的操纵区与RRTRES的亲和力最高,Kd值约为lpM;当结合位点为TTAC时,平均Kd值为3pM:当结合位点为 TTCC时,Kd值在5-lOpM之间。天然噬菌体434阻遏蛋白与其操纵区的亲和力的Kd值在nM数量级,与之相比,所筛选操纵区的亲和力明显提高。此外,亲和力大小还受到结合位点两侧的碱基的影响,特别是5'位碱基的影响。 表达纯化同源双突变的单链阻遏蛋白RTRESRTRE'根据RTRES的以上识别特一点,设计了一系列新的操纵区序列,它们的共有序列为GTAAGAAARNTTACN,或GGAAGAAARNTTCCN,并测定它们与RTRES RTRE之间的结合特异性。结果表明,它们可被RTRES RTRES特异识别,且亲和力也很高,Kd值在5-40pM之间。其中GTAAGAAAGTTTACG与RTRES RTRES之间结合的Kd值约为5pM。同样,表达了异源双突变的单链阻遏蛋白R*RTRES,然而它与 设计的相关操纵区的亲和力并不很高,Kd值约为lOOpM。利用本工作中的随机筛选和合理设计的原则,得到了新的具有特异性识别和高亲和力的蛋白一DNA相互作用。这个方法可望用于其他DBP的新的结合特异性的筛选。 二. 非同位素的方法筛选单链阻遏蛋白的最佳DNA结合序列初探 克隆和表达了带半胱氨酸尾的单链阻遏蛋白,利用已包被了马来酰胺的活性板可以与自由巯基结合的特性,将蛋白固定在活性板表面。体外筛选RTRES RTRES的最佳DNA结合序列,得到了一些与RTRES RTRES结合的序列,但Kd值nM数量级。此方法需进一步优化。
Resumo:
当前分子生物学的方法以惊人的速度渗透到生命科学研究的各个领域。植物对不断变化的环境逐步适应的过程中,积累了丰富的遗传多样性。与此同时,人类活动空间的不断扩大已经严重威胁到其他生命的生存和繁衍,越来越多的物种以越来越快的速度在我们还没有来得及认识它们时就已经永远地消失了。加快物种鉴定和保护的步伐就必须发展更多能充分揭示物种遗传多样性的实验技术,从具有丰富遗传多样性的野生资源中寻找到更多能够服务于人类可持续发展的基因资源。本文以杨树杂交后代过氧化物同工酶和RAPD分析为基础,论证了我们改进的RAPD方法用于遗传分析的可行性。在前期工作的基础上,进一步测定了野大豆自然群体的耐盐性变异,并且用微卫星和RAPD分析的方法研究分子标记与DXA变异、植株耐盐性之间的关系。对四个可能与抗盐性有关的RAPD片段进行克隆、测序,并进行序列比较。由此得出以下结论: 1、在本文的实验条件下,杨树同工酶和RAPD分析均表明,RAPD标记在亲本及其杂交后代中性状比例符合孟德尔遗传规律,尽管有时也会出现遗传负载等机制引起的基因分布扭曲现象。 2、初步研究了个体发育阶段和环境条件对植株耐盐性的影响。结果表明,植物耐盐性不仅仅与外界的盐度有关,而且受发育阶段和其它环境条件(如,温度)的影响。但也发现了某些个体在各种条件下都具有较高的耐盐性,而且,不易受到其它环境条件的影响。 3、微卫星标记的结果表明,10对引物中的8对引物共检测到时17个等位基因,平均每对引物2.125个等位基因。本文的实验条件下,双核苷酸和三核苷酸的引物对扩增产物都没有出现“ghosts"条带或“打滑”现象。 4、有4个RAPD标记可能与野大豆群体的耐盐性有关,分别是OPCO8460bp、OPCO8213bp、OPCO2690bp、以及OPCO5270bp。测序结果与GenBank中的序列作同源性比较,结果显示,OPCO2_(690bp)与小麦、松树等植物的吉普赛性的逆转录转座子的部分区域(24--53)有很高的同源性(86-89%)。此外,OPCO2690bp与栽培大豆胞质谷氨酰胺合成酶(gs15)基因的启动子有高达95%的同源性。 5、本文实验条件下,RAPD扩增产物在限制性内切酶消化后,消化产物的多态性未见增大,也没有发现与耐盐性相关的多态位点。 6、野大豆自然群体DNA变异的研究中也可以应用SWAPP方法。
Resumo:
低能离子束的诱变效应首先由我国科学家发现并将其广泛应用于育种实践,但是离子注入诱导DNA变异的研究结果主要是以微生物离体质粒DNA为材料获得的,以活体高等生物为材料的研究尚未见报道。 我们以30 keV N+(注入剂量80×1015 ions/cm2)注入拟南芥后获得的稳定突变体T80II为实验材料,对突变体植株进行了RAPD标记,并将T80II和对照部分RAPD特异条带进行克隆测序和DNA序列分析。结果显示,在可分辨的总计397个RAPD条带中,T80II株系中有52个条带表现出差异,包括条带的缺失和增加,条带变异率为13.1%;克隆的T80II序列中,平均每16.8个碱基出现一个碱基变异位点,表现出较高频率的碱基突变。碱基突变的类型包括碱基的颠换、转换、缺失、插入等。在检测到的275个碱基突变中,主要是单碱基置换(97.09%),碱基缺失或者插入的比例较小(2.91%)。在碱基置换中,转换的频率(66.55%)高于颠换的频率((30.55%)。此外,构成DNA的四种碱基均可以被离子束辐照诱发变异,而且每一种碱基都可以被其它三种碱基所替换,但是胸腺嘧啶(T)的辐射敏感性要高于其它三种碱基。通过分析突变碱基周边序列,对低能N+离子注入拟南芥突变体引发的碱基突变热点进行了讨论。 另外,低能离子注入诱变获得的突变体特异表达基因的克隆方面也没有报道。我们以突变体T80II作为实验材料,用PCR增效的减法杂交技术构建了T80II特异表达的cDNA减法文库,克隆特异表达的cDNA片段,并对其中1个与14-3-3 protein GF14 nu (GRF7) gene有部分同源性、长712 bp的cDNA片段进行了讨论。我们的研究证明通过减法杂交技术克隆低能离子诱发的突变体特异表达的cDNA是可能的,这为低能离子注入技术在分子生物学上的应用开辟了一个新思路。
Resumo:
A total of 1006 king mackerel (Scomberomorus cavalla) representing 20 discrete samples collected between 1996 and 1998 along the east (Atlantic) and west (Gulf) coasts of Florida and the Florida Keys were assayed for allelic variation at seven nuclear-encoded microsatellites. No significant deviations from Hardy-Weinberg equilibrium expectations were found for six of the microsatellites, and genotypes at all microsatellites were independent. Allele distributions at each microsatellite were independent of sex and age of individuals. Homogeneity tests of spatial distributions of alleles at the microsatellites revealed two weakly divergent “genetic” subpopulations or stocks of king mackerel in Florida waters—one along the Atlantic coast and one along the Gulf coast. Homogeneity tests of allele distributions when samples were pooled along seasonal (temporal) boundaries, consistent with the temporal boundaries used currently for stock assessment and allocation of the king mackerel resource, were nonsignificant. The degree of genetic divergence between the two “genetic” stocks was small: on average, only 0.19% of the total genetic variance across all samples assayed occurred between the two regions. Cluster analysis, assignment tests, and spatial autocorrelation analysis did not generate patterns that were consistent with either geographic or spatial-temporal boundaries. King mackerel sampled from the Florida Keys could not be assigned unequivocally to either “genetic” stock. The genetic data were not consistent with current spatial-temporal boundaries employed in stock assessment and allocation of the king mackerel resource. The genetic differences between king mackerel in the Atlantic versus those in the Gulf most likely stem from reduced gene flow (migration) between the Atlantic and Gulf in relation to gene flow (migration) along the Atlantic and Gulf coasts of peninsular Florida. This difference is consistent with findings for other marine fishes where data indicate that the southern Florida peninsula serves (or has served) as a biogeographic boundary.
Resumo:
Independent molecular markers based on mitochondrial and nuclear DNA were developed to provide positive identification of istiophorid and xiphiid billfishes (marlins, spearfishes, sailfish, and swordfish). Both classes of markers were based on amplification of short segments (<1.7 kb) of DNA by the polymerase chain reaction and subsequent digestion with informative restriction endonucleases. Candidate markers were evaluated for their ability to discriminate among the different species and the level of intraspecific variation they exhibited. The selected markers require no more than two restriction digestions to allow unambiguous identification, although it was not possible to distinguish between white marlin and striped marlin with any of the genetic characters screened in our study. Individuals collected from throughout each species’ range were surveyed with the selected markers demonstrating low levels of intraspecific character variation within species. The resulting keys provide two independent means for the forensic identification of fillets and for specific identification of early life history stages.
Resumo:
We used allozyme, microsatellite, and mitochondrial DNA (mtDNA) data to test for spatial and interannual genetic diversity in wall-eye pollock (Theragra chalcogramma) from six spawning aggregations representing three geographic regions: Gulf of Alaska, eastern Bering Sea, and eastern Kamchatka. Interpopulation genetic diversity was evident primarily from the mtDNA and two allozyme loci (SOD-2*, MPI*). Permutation tests ˆindicated that FST values for most allozyme and microsatellite loci were not significantly greater than zero. The microsatellite results suggested that high locus polymorphism may not be a reliable indicator of power for detecting population differentiation in walleye pollock. The fact that mtDNA revealed population structure and most nuclear loci did not suggests that the effective size of most walleye pollock populations is large (genetic drift is weak) and migration is a relatively strong homogenizing force. The allozymes and mtDNA provided mostly concordant estimates of patterns of spatial genetic variation. These data showed significant genetic variation between North American and Asian populations. In addition, two spawning aggregations in the Gulf of Alaska, in Prince William Sound, and off Middleton Island, appeared genetically distinct from walleye pollock spawning in the Shelikof Strait and may merit management as a distinct stock. Finally, we found evidence of interannual genetic variation in two of three North American spawning aggregations, similar in magnitude to the spatial variation among North American walleye pol-lock. We suggest that interannual genetic variation in walleye pollock may be indicative of one or more of the following factors: highly variable reproductive success, adult philopatry, source-sink metapopulation structure, and intraannual variation (days) in spawning timing among genetically distinct but spatially identical spawning aggregates.
