中国极小种群野生植物保护理论与实践研究进展

极小种群野生植物大都分布范围狭窄、个体数量稀少且自然更新困难, 面临随时灭绝的风险, 迫切需要拯救性保护。极小种群野生植物这一概念自提出以来受到了保护生物学领域的广泛关注, 已成为当前中国生物多样性保护的一个热点方向。我国于2010年正式启动实施极小种群野生植物拯救保护工程, 并开展了大量的保护研究和实践。以“extremely small population*”和“plant”为检索词在Web of Science进行了主题检索, 以“极小种群”和“植物”为检索词在中国知网进行了主题检索, 对获取的的学术期刊论文、学位论文和会议论文进行了梳理。本文从极小种群野生植物种群、群落及生境调查与监测、适应性、遗传多样性、繁殖生物学、濒危机制、动态模型6个方面对近年来极小种群野生植物的理论研究工作进行了较为系统的综述。在此基础上, 从就地保护、迁地保护与种质资源保存、野外回归、人工繁育、标准化体系5个方面回顾了极小种群野生植物保护实践及取得的进展。基于极小种群野生植物保护理论与实践研究现状, 我们建议在极小种群野生植物未来保护工作中不断调整和完善保护名录, 加强种群结构的观测和预测、小种群形成和恢复机制的针对性研究以及特定物种的长期系统性研究, 同时促进这一概念在国际上的推广。希望本文能为国家生物多样性保护和生态文明建设提供参考。     

Ras-related proteins (Rab) are key proteins related to male fertility following a unique activation mechanism

Ras-related protein Rab (Rab) proteins, member of Ras superfamily of monomeric G proteins, are well known key regulators of intracellular vesicular transport. Recently, it has been reported that Rab 2A and 3A are related to acrosomal exocytosis in spermatozoa and Rab 2A can be used to fertility-related biomarker in male. However, the role and mechanism of Rab proteins in spermatozoa has not been fully understood yet. Therefore, the study to analyze the expression and location of various Rab proteins in spermatozoa is required to understand the role and mechanism of Rab proteins in spermatozoa. In present study, to analyze the expression level and location of various Rab proteins (Rab 2A, Rab3A, Rab4, Rab5, Rab8A, Rab9, Rab11, Rab14, Rab25, Rab27A, and Rab34) and Rab protein regulators (RabGAP, RabGDI, RabGEF) in spermatozoa following capacitation, immunofluorescence and western blot analysis were performed. All of 11 Rab proteins were expressed in acrosomal region and tail of spermatozoa. Furthermore, all Rab proteins and Rab protein regulators, except RabGAP, have decreased expression patterns after capacitation. Taken together, Rab proteins were located in sperm head and tail. In addition, expression patterns of Rab proteins in spermatozoa were altered following capacitation. Therefore, our results suggested that Rab proteins may be key proteins related with capacitation as well as playing important role with uniquely activation pathway for male fertility.     

RAL GTPases Drive Intestinal Stem Cell Function and Regeneration through Internalization of WNT Signalosomes

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Bipartite Topology of Treponema pallidum Repeat Proteins C/D and I: OUTER MEMBRANE INSERTION,TRIMERIZATION, AND PORIN FUNCTION REQUIRE A C-TERMINAL β-BARREL DOMAIN*

We previously identified Treponema pallidum repeat proteins TprC/D, TprF, and TprI as candidate outer membrane proteins (OMPs) and subsequently demonstrated that TprC is not only a rare OMP but also forms trimers and has porin activity. We also reported that TprC contains N- and C-terminal domains (TprC^N and TprC^C) orthologous to regions in the major outer sheath protein (MOSP^N and MOSP^C) of Treponema denticola and that TprC^C is solely responsible for β-barrel formation, trimerization, and porin function by the full-length protein. Herein, we show that TprI also possesses bipartite architecture, trimeric structure, and porin function and that the MOSP^C-like domains of native TprC and TprI are surface-exposed in T. pallidum, whereas their MOSP^N-like domains are tethered within the periplasm. TprF, which does not contain a MOSP^C-like domain, lacks amphiphilicity and porin activity, adopts an extended inflexible structure, and, in T. pallidum, is tightly bound to the protoplasmic cylinder. By thermal denaturation, the MOSP^N and MOSP^C-like domains of TprC and TprI are highly thermostable, endowing the full-length proteins with impressive conformational stability. When expressed in Escherichia coli with PelB signal sequences, TprC and TprI localize to the outer membrane, adopting bipartite topologies, whereas TprF is periplasmic. We propose that the MOSP^N-like domains enhance the structural integrity of the cell envelope by anchoring the β-barrels within the periplasm. In addition to being bona fide T. pallidum rare outer membrane proteins, TprC/D and TprI represent a new class of dual function, bipartite bacterial OMP.     

小型哺乳动物的繁殖投入与繁殖成功率

动物的繁殖活动关系到整个种群的生存与灭绝, 繁殖投入和繁殖成功率是繁殖生态学研究的重要内容。从繁殖投入的划分入手, 综述了小型哺乳动物的繁殖投入和繁殖成功率之间的关系及其影响因素、分子生物学技术在繁殖生态学中的应用等, 阐述了小型哺乳动物能够根据自身的状态调整每次繁殖活动中的时间投入和能量分配, 采取不同的繁殖对策。这些繁殖对策是长期自然选择的结果, 其目的都是为了最大限度地提高自身的适合度。并且指出分子生物学技术在繁殖生态学中的应用将大大加快这一研究领域的快速发展。     

COMP-Ang1 inhibits apoptosis as well as improves the attenuated osteogenic differentiation of mesenchymal stem cells induced by advanced glycation end products

Background

In the present study, we have investigated the possibility that cartilage oligomeric matrix protein angiopoietin1 (COMP-Ang1), important factor in angiogenesis, osteogenesis and the survival of mesenchymal stem cells (MSCs) through the Ang1/Tie2 pathway has beneficial effects on osteogenic differentiated cells (ODCs) from MSCs treated by advanced glycation end products (AGE), which are pathological factors of diabetes.

Methods

Primary culture of MSCs was used. For comparison analysis of AGE and COMP-Ang1 effects, we performed cell viability assay with each treated variety concentration for 24 h. Apoptosis rate and Caspase-3 activity were measured by each ELISA assay. To make sure with Ang1/Tie2 pathway, we performed small interfering RNA transfected to MSCs. Real-time RT-PCR was performed to identify ODCs marker genes. Immunoblotting was used to evaluate the expression of Tie2, AKT, p38 and ERK.

Results

Our results clearly demonstrate that COMP-Ang1 upregulates the phosphorylation of AKT and p38 by activating the Ang1/Tie2 signaling pathway, indicating that COMP-Ang1 affects both AGE-induced apoptosis and the attenuated osteogenic differentiation of MSCs through the p38/MAPK and PI3K/AKT pathways.

Conclusions

COMP-Ang1 improves cell viability and differentiation function of ODCs against AGE via Ang/Tie2 signaling pathway.

General significance

Our results suggest the potential importance of COMP-Ang1 as a new therapy for impaired bone formation that is associated with diabetes and advanced age.     

Spotting the right location— imaging approaches to resolve the intracellular localization of invasive pathogens

Background

A common strategy of microbial pathogens is to invade host cells during infection. The invading microbes explore different intracellular compartments to find their preferred niche.

Scope of Review

Imaging has been instrumental to unravel paradigms of pathogen entry, to identify their exact intracellular location, and to understand the underlying mechanisms for the formation of pathogen-containing niches. Here, we provide an overview of imaging techniques that have been applied to monitor the intracellular lifestyle of pathogens, focusing mainly on bacteria that either remain in vacuolar-bound compartments or rupture the endocytic vacuole to escape into the host's cellular cytoplasm.

Major Conclusions

We will depict common molecular and cellular paradigms that are preferentially exploited by pathogens. A combination of electron microscopy, fluorescence microscopy, and time-lapse microscopy has been the driving force to reveal underlying cell biological processes. Furthermore, the development of highly sensitive and specific fluorescent sensor molecules has allowed for the identification of functional aspects of niche formation by intracellular pathogens.

General Significance

Currently, we are beginning to understand the sophistication of the invasion strategies used by bacterial pathogens during the infection process- innovative imaging has been a key ingredient for this.This article is part of a Special Issue entitled Nanotechnologies - Emerging Applications in Biomedicine.     

siRNA抑制哺乳动物细胞内Rab9 GTPase表达的研究

构建Rab9 GTPase siRNA表达载体,观察siRNA对哺乳动物细胞内Rab9 GTPase表达的抑制作用,为应用Rab9 GTPase siRNA表达载体进行抗麻疹病毒感染研究奠定基础。根据Rab9 GTPase基因的mRNA序列设计合成2对靶向Rab9 GTPase基因的寡核苷酸,克隆到表达载体pSUPER.neo EGFP,通过双酶切和序列分析对重组表达载体进行鉴定。将鉴定为阳性的重组表达载体转染B95a细胞株,通过逆转录聚合酶链反应(RT-PCR)和免疫印迹技术(Western-blot)检测B95a细胞内Rab9 GTPase mRNA和蛋白的表达水平。双酶切和序列分析表明成功构建了Rab9 GTPase siRNA表达载体,RT-PCR和Western-blot技术实验表明重组表达载体可显著抑制B95a细胞内Rab9 GTPase mRNA和蛋白的表达(最高抑制率分别为89.4%±0.5%和87.6%±0.7%),而对照组则没有变化。结果表明,成功构建了Rab9 GTPase siRNA表达载体,该表达载体可有效地抑制Rab9 GTPase在哺乳动物细胞内的表达。     

The complete nucleotide sequence of the mitochondrial genome of the oriental fruit fly, Bactrocera dorsalis (Diptera: Tephritidae)

The complete mitochondrial genome of the oriental fruit fly Bactrocera dorsalis s.s. has been sequenced, and is here described and compared with the homologous sequences of Bactrocera oleae and Ceratitis capitata. The genome is a circular molecule of 15,915 bp, and encodes the set of 37 genes generally found in animal mitochondrial genomes. The structure and organization of the molecule is typical and similar to the two closely related species B. oleae and C. capitata, although it presents an interesting case of putative intra-molecular recombination. The relevance of the growing comparative dataset of tephritid complete mitochondrial genomes is discussed in relation to the possibility to develop robust assays for species discrimination in quarantine and agricultural monitoring practices, as well as basic phylogeography/population genetic studies.