Tag retention,wound healing,and subsequent reproductive history of southern right whales following satellite‐tagging

This paper presents data from 48 resightings of 16 southern right whales that were satellite‐tagged on the South African coast in September 2001, up to and including 2012. Tag performance in terms of number of days with locations received was significantly higher in males than females, and lowest in cows with calves, and attributed to behavioral differences leading to variable degrees of antenna damage. Resightings occurred from 4 to 4,054 d after tagging: tags were retained in all whales seen within 27 mo, but were apparently shed in all but one individual seen within 36 mo of tagging. The exception was a whale that still had the tag present 11 yr after tagging. Healing at the tag site occurred gradually and within 5 yr of tagging (and 2 yr after tag shedding). No significant difference in the subsequent frequency of calving was detected between 12 tagged and 382 untagged females photographed contemporaneously, and although statistical power was low, a 21% or greater reduction in calving rate in tagged females would seem incompatible with the observations. The death of one female 3 yr after tagging was more likely attributable to a ship strike on an animal debilitated by a prolapsed uterus.     

Interactome Analysis of Human Phospholipase D and Phosphatidic Acid-Associated Protein Network

Mammalian phospholipase D (PLD) enzyme family consists of six members. Among them, PLD1/2/6 catalyzes phosphatidic acid (PA) production, while PLD3/4/5 has no catalytic activities. Deregulation of the PLD-PA lipid signaling has been associated with various human diseases including cancer. However, a comprehensive analysis of the regulators and effectors for this crucial lipid metabolic pathway has not been fully achieved. Using a proteomic approach, we defined the protein interaction network for the human PLD family of enzymes and PA and revealed diverse cellular signaling events involving them. Through it, we identified PJA2 as a novel E3 ubiquitin ligase for PLD1 involved in control of the PLD1-mediated mammalian target of rapamycin signaling. Additionally, we showed that PA interacted with and positively regulated sphingosine kinase 1. Taken together, our study not only generates a rich interactome resource for further characterizing the human PLD-PA lipid signaling but also connects this important metabolic pathway with numerous biological processes.     

充分利用EST数据库资源

表达序列标签(EST）数据库作为一种重要的基因组数据库,已成为新基因的发现、基因表达及重组蛋白表达等研究的有力分子生物学工具.介绍了如何充分利用EST数据库.     

小麦种子基因的表达序列标签分析

以授粉后12 d的小麦(Triticum aestivum L.)种子为材料,构建起cDNA文库.从中随机挑选10 000个克隆,利用Biomek 2000核酸工作站制成高密度cDNA阵列.然后分别以未受精子房、胚和胚乳中提取的RNA为模板,反转录合成探针与膜杂交,进行差示筛选.根据筛选结果,选取800个在胚、胚乳或胚和胚乳中表达的克隆进行表达序列标签(EST)分析,鉴定出216个不同的基因序列.其中24个ESTs属于已知的小麦基因;122个ESTs为推测的小麦新基因,它们编码的产物与种子贮藏蛋白或与生化代谢、发育等其他的生物学过程有关;70个ESTs的序列特征尚未确定.本研究为研究种子发育和小麦品质改良等提供了基础资料.     

林木遗传连锁图谱构建研究进展与发展方向

本文就目前国内外林木连锁遗传图谱领域的研究进展进行了综述,指出了该领域研究中存在的主要问题,即一方面是作图个体的数量有限,另一方面是采用的标记以随机标记为主,导致了建成的图谱以及利用图谱获得的数量性状基因位点（QTLs）信息具有杂交组合特异性,造成了QTLs的可信度和在林木遗传改良以及标记辅助选择中的实用性降低等现象。针对存在的问题,讨论了根据林木生物学特点选择合适遗传标记的意义,指出进行林木比较作图研究的重要性和必要性。文中接着较为详尽地介绍了国外重要林木表达序列标签（EST）测序项目的研究进展,论述了功能已知和种间高度保守的表达序列标签多态性（ESTP）标记的由来,阐述了获得ESTP标记的主要方法,并指出应当利用ESTP标记进行林木遗传图谱构建、QTL定位和比较作图的研究。文中最后讨论了未来林木遗传图谱构建和QTL定位研究的发展方向,并探讨了我国在该领域取得重大进展的突破口,指出我国应首先进行杨树尤其是中国乡土杨树树种该方面的研究。 Abstract:The research progress in genetic linkage map construction of forest tree species both at home and abroad were reviewed in the paper.Two main problems involved in the field were discussed.One was the limitation of the number of individuals of mapping populations and the other was the random markers mostly employed by the majority of studies.These problems have resulted in crossing combination specificity in the constructed maps and the QTLs located on the basis of the maps.As a result,the QTLs discovered up to now have low credibility and poor practicability in marker-assisted selection.Therefore considering the biological characteristics of forest tree species,the selection of the most suitable genetic markers is crucial to obtain a high quality genetic linkage map,and it is both important and necessary to carry out comparative genetic mapping.Progress in the ongoing expressed sequence tag (EST) sequencing projects were summarized and EST polymorphism (ESTP),the most informative and highly conservative marker with known function,as well as the main ESTP detection techniques were elaborated.It was pointed out that ESTP markers should be integrated into the present studies of genetic linkage map construction,QTL mapping and genome comparative mapping.Finally the future prospects in the fields of genetic linkage map and QTL mapping were discussed.In China,Such studies around Populus,especially in the local Populus species should make a breakthrough in the related fields.     

Comparison between gene expression of conidia and germinating phase in Trichophyton rubrum

Trichophyton rubrum is a dominating superficial dermatophyte, whose conidial germination is correlated to pathopoiesis and a highly important developmental process. To investigate the changes of physiology, biochemistry and cytology during the germination, we selected 3364 function identified ESTs from T. rubrum cDNA library to construct cDNA microarrays, and compared the gene expression levels of conidia and germinating phase. Data analysis indicated that 335 genes were up-regulated during the germination, which mainly encoded translated, modified proteins and structural proteins.The constituents of cell wall and cell membrane were synthetized abundantly, suggesting that they are the foundation of cell morphogenesis. The ingredients of the two-component signal transduction system were up-regulated, presuming that they were important for the conidial germination. Genes of various metabolic pathways were expressed prosperously, especially the genes that participated in glycolysis and oxidative phosphorylation were up-regulated on the whole, demonstrating that in the environment with sufficient oxygen and glucose, conidia obtained energy through aerobic respiration.This paper provides important clues which are helpful to understanding the changes in gene expression, signal conduction and metabolism characteristics during T. rubrum conidial germination, and possess significant meaning to the study of other superficial dermatophytes.     

Retention of visible implant tags by juvenile brown trout

The retention and readability of visible implant (VI) tags were evaluated in juvenile brown trout. The tags were implanted in the adipose eyelid tissue posterior to the left eye, in a total of 6697 fish in 18 groups. During the first year, tag retention increased with tagging experience, from 58 to 64% in 3–summer–old fish and from 86 to 96% in 4–summer–old fish. The effect of fish size at tagging on tag loss was clear in the 3–summer–old groups in 1991 (ANOVA, P = 0.00001). Tag retention in 3–year–old and 4–summer–old fish in 1992 and 1993 varied from 96 to 99% and the handling of the fish after tagging affected retention significantly ( t –test, P = 0.0002), the average being 98.7% for those transposed by submerging and 96.5% in those transposed by dropping. After inspection the fish were released into a natural environment. On recapture after 6 months or more the red tags (faded almost to white) and yellow tags (originally close to white) were difficult to distinguish. No infection or tissue damage was found after either inspection or stocking.     

Functional genomics: going forwards from the databases

Extrapolating systematically from gene sequence to function is undoubtedly the major challenge facing industry and academia alike as we approach the end of the millennium. Many electronic and laboratory approaches are being developed to meet this challenge but the rate of evolution of these is not keeping pace with the speed of sequence generation.     

Bioinformatics: from genome data to biological knowledge

Recently, molecular biologists have sequenced about a dozen bacterial genomes and the first eukaryotic genome. We can now obtain answers to detailed questions about the complete set of genes of an organism. Bioinformatics methods are increasingly used for attaching biological knowledge to long lists of genes, assigning genes to biological pathways, comparing the gene sets of different species, identifying specificity factors, and describing sets of highly conserved proteins common to all domains of life. Substantial progress has recently been made in the availability of primary and added-value databases, in the development of algorithms and of network information services for genome analysis. The pharmaceutical industry has greatly benefited from the accumulation of sequence data through the identification of targets and candidates for the development of drugs, vaccines, diagnostic markers and therapeutic proteins.     

The Diphtheria Toxin Channel-forming T Domain Translocates Its Own NH2-Terminal Region Across Planar Bilayers

The T domain of diphtheria toxin, which extends from residue 202 to 378, causes the translocation of the catalytic A fragment (residues 1–201) across endosomal membranes and also forms ion-conducting channels in planar phospholipid bilayers. The carboxy terminal 57-amino acid segment (322–378) in the T domain is all that is required to form these channels, but its ability to do so is greatly augmented by the portion of the T domain upstream from this. In this work, we show that in association with channel formation by the T domain, its NH₂ terminus, as well as some or all of the adjacent hydrophilic 63 amino acid segment, cross the lipid bilayer. The phenomenon that enabled us to demonstrate that the NH₂-terminal region of the T domain was translocated across the membrane was the rapid closure of channels at cis negative voltages when the T domain contained a histidine tag at its NH₂ terminus. The inhibition of this effect by trans nickel, and by trans streptavidin when the histidine tag sequence was biotinylated, clearly established that the histidine tag was present on the trans side of the membrane. Furthermore, the inhibition of rapid channel closure by trans trypsin, combined with mutagenesis to localize the trypsin site, indicated that some portion of the 63 amino acid NH₂-terminal segment of the T domain was also translocated to the trans side of the membrane. If the NH₂ terminus was forced to remain on the cis side, by streptavidin binding to the biotinylated histidine tag sequence, channel formation was severely disrupted. Thus, normal channel formation by the T domain requires that its NH₂ terminus be translocated across the membrane from the cis to the trans side, even though the NH₂ terminus is >100 residues removed from the channel-forming part of the molecule.