基因型值多次聚类法构建作物种质资源核心库

采用合适的遗传模型无偏预测基因型值,用基因型值进行聚类分析,采用马氏距离计算遗传材料间的遗传距离,并用不加权类平均法（ＵＰＧＭＡ）进行聚类,根据树型图,从遗传变异相似的每组二个遗传材料中随机选取一个遗传材料,如组内只有一个遗传材料,则选取该遗传材料,对所取的所有遗传材料再次聚类、取样,直至所取遗传材料的数量为总遗传的２０％￣３０％,这些遗传材料作迷为核心聚类。用方差同质性测验、均值ｔ测验评核心资源     

植物种质群体遗传结构改变的测度

本文旨在探讨植物种质资源保存中由于人为和自然缘故导致遗传结构改变的评价指标和评价方法.在介绍植物种质资源保存研究一些基本概念的基础上,归纳了测度种质库(收集品)遗传潜势的6种遗传多样性统计指标,包括同一变异层次的类型数、类型分布均衡度、遗传相似性与遗传距离、遗传方差与遗传变异系数、多元变异指数以及亲本系数.指出若无遗传丰富度相伴,单有遗传离散度并未提供遗传多样性的完整测度.探讨了人为条件导致植物种质资源遗传结构改变的遗传流失、环境胁迫所致植物种质资源遗传结构改变的遗传脆弱性和种子扩繁所引发的植物种质资源遗传结构改变的遗传漂变和遗传漂移等的统计指标.文末给出了自花授粉植物和异花授粉植物群体适宜样本容量研究的个例.     

水稻SSR标记的遗传多样性研究进展

本文从SSR标记优点和适用于研究水稻遗传多样性入手,综述了SSR标记在水稻核心种质构建与评价、遗传结构、稻种起源演化等方面的研究进展。总结了水稻遗传多样性的地带性特征（云南是中国稻种资源的最大遗传多样性中心和优异种质的富集地;西南稻区粳稻品种遗传多样性最丰富;南方稻区粳稻品种的遗传多样性高于北方粳稻遗传多样性）、遗传多样性与生态地理位置密切相关、目前水稻品种遗传基础狭窄、多样性降低等特征,分析了遗传多样性成因及影响因素,特别指出了育种行为对遗传多样性的影响,并针对当前水稻品种遗传多样性较低的问题提出了对策。     

细胞质遗传并非都是母系遗传

细胞质遗传一般表现为具母系遗传的特征。随着ＤＮＡ分子标记技术的发展和应用,人们已发现在动物及植物中均存在有低频的线粒体ＤＮＡ单亲父系遗传及双亲遗传的现象,对质体ＤＮＡ遗传的研究表明,被子植物的质体ＤＮＡ大多表现为母系遗传。而裸子植物的质体ＤＮＡ则主要表现为父系遗传的方式,同时也出现存在其它的遗传规律。     

情感性障碍遗传因素与遗传方式的研究A

本文对205例情感性障碍患者的遗传因素与遗传方式作了研究．分析了先证者的家族遗传史,各级亲属的患病率及环境因素的作用,认为遗传因素在悄感性障碍的病因中具有重要的意义．同时,通过统计分析,指出情感性障碍的遗传方式为多基因遗传,其加权午均遗传率为78.99%.     

遗传病系谱的特点

系谱是指在调查某种遗传病患者家族成员的发病情况后,按一定形式绘成的图解。(?)根据致病基因所在的染色体种类不同,可以分为下列几种情况:常染色体遗传显性遗传隐性遗传性染色体遗传显性遗传隐性遗传无论何种遗传病都有自己的特点,根据这些特点可以判断出某种遗传病的遗传方式。     

“遗传的基本规律”单元复习的组织

高中生物学所讲述的遗传的基本规律包括基因的分离定律、自由组合定律、伴性遗传定律以及细胞质遗传的特点。其中,基因的分离定律、自由组合定律和伴性遗传定律揭示了细胞核遗传的一般规律,与细胞质遗传呈现并列平行关系。     

果蝇眼色遗传及基因漫谈

通过果蝇复眼颜色遗传的几个遗传规律来说明基因之间的一些相互关系,既要能分解简化遗传规律,又要综合看待遗传规律,对遗传的复杂性要有进一步的认识。     

“《遗传学报》创刊30周年学术研讨会”征文通知

1.主办单位:中国遗传学会,中国科学院遗传与发育生物学研究所,东南大学 承办单位:《遗传学报》、《遗传》杂志编辑室,东南大学医学院遗传学研究中心2.大会主席:中国遗传学会理事长赵寿元;《遗传学报》、《遗传》杂志主编朱立煌 东南大学校长　顾冠群 大会副主席:《遗传学报》副主编　陈 竺、吴常信、李家洋、张启发 中国科学院遗传与发育生物学研究所副所长　薛勇彪 东南大学副校长　浦跃朴     

分子遗传保护研究进展

介绍了遗传保护的内涵和遗传保护的途径及存在的问题,从遗传多样性检测、种群内遗传变异及进化分化的鉴别、就地或移地保护物种的繁殖与遗传保护、遗传结构地理差异、种群大小的遗传基础与保护等方面综述了遗传保护研究的进展。     

Different cytoskeletal organization in two maturation stages of Discoglossus pictus (Anura) oocytes: thickness and stability of actin microfilaments and tropomyosin immunolocalization

In Discoglossus pictus oocytes, the germinative area (GA) contains long and irregular microvilli where actin microfilaments are located. In the egg, the funnel-shaped dimple that originates by invagination of the GA is present. In the dimple both microvilli and microfilament bundles have a very orderly appearance. This report extends previous observations (Campanella and Gabbiani, Gamete Res 3:99-114, 1980) and shows that GA microfilaments are thinner (36 A average) than dimple microfilaments (60 A average), as measured in ultrathin section. Moreover, the interfilament distance is smaller in GA bundles than in the dimple bundles. To get an insight into actin organization in oocytes and eggs, we used an actin-depolymerizing factor (ADF) in which cryostat sections were incubated prior to immunofluorescent staining with antiactin antibodies. The microfilaments of the GA microvilli and partially of the oocyte cortex are resistant to ADF when compared to those in the dimple and the rest of the egg cortex. We also investigated immunocytochemically the presence of tropomyosin and found that this protein is localized in the dimple and in the cortex of oocytes and eggs but is absent in the GA.     

Cytoskeletal and contractile proteins in coelomic oocytes,unfertilized and fertilized eggs of discoglossus pictus (Anura)

The distribution of actin, myosin, and tubulin has been investigated in coelomic oocytes, unfertilized and fertilized eggs of Discoglossus pictus utilizing: (1) immunofluorescence; (2) electron microscopy; (3) incubation with heavy meromyosin (HMM), and (4) SDS-polyacrylamide gel electrophoresis (PAGE). In coelomic oocytes, the germinative area (GA) has long, irregular microvilli containing microfilaments. In the rest of the oocyte, the microvilli are shallow. During the transit of the oocyte in the oviduct, a dimple forms by the invagination of the GA. A palisade of microfialment bundles is present in the finger-shaped microvilli of the dimple and extends for about 10 μm in the cytoplasm. In the rest of the egg, microvilli are absent and only random filaments appear in the cortex. Following HMM incubation, the dimple microfilaments are decorated with arrowheads pointing toward the bulk of the cytoplasm. SDS-PAGE of egg extracts shows bands co-migrating with actin (43K), pyruvate kinase (57K), and phosphorylase (94K). As result fertilization, the pattern of microfilament bundles in the dimple disappers in parallel with the dimple invergination itself. Generally, the entire oocyte cortex is positive to immunofluorescent staining with anti-actin, antimyosin, and antitubulin antibodies. However, the pattern of distribution and intensity of immunofluorescent staining changes for each antiserum, during different stages. It is concluded that a contractile system is present in Discoglossus eggs, and it is particularly developed in the dimple. The dimple is probably a major compartment for the storage of unpolymerized tubulin.     

A highly localized activation current yet widespread intracellular calcium increase in the egg of the frog, Discoglossus pictus

Sperm entry in the egg of the painted frog, Discoglossus pictus, occurs only at a specialized region of the animal hemisphere called the animal dimple, a structure not found in other species of frog. An extracellular vibrating electrode was used to measure the activation current to determine if the ion channels that open to generate the fertilization potential are localized in this region. Eggs that were activated by microinjecting inositol-1,4,5-trisphosphate (Ins(1,4,5)P3) exhibited activation potentials very similar to those of fertilized eggs. There was a delay between the time of Ins(1,4,5)P3 injection and the initiation of the activation potential that was proportional to the distance between the site of the activating stimulus and the animal dimple, similar to the delay previously observed in prick-activated eggs (R. Talevi, B. Dale, and C. Campanella (1985). Dev. Biol. 111, 316-323). The delay lasted 30 sec when the stimulus site was 20 degrees (300 micron) from the animal dimple and 14 min when it was 150 degrees C from the dimple. Once the activation potential was initiated, there was an excellent temporal correlation between the time of depolarization and the time of the first detectable current entering the dimple region. This inward current was typically 60 microA/cm2 in amplitude and was found only in the central 200 micron of the dimple region. The outward current was distributed over the remainder of the egg surface and was much smaller in amplitude. The activation current was carried by Cl- efflux in the animal dimple region, and was reduced by DIDS and reversed by high external Cl- or I-. The occurrence of inward current only at the dimple region indicates that Cl- channels which open to produce the activation potential are localized there. Using Ca2+-specific microelectrodes, we found that [Ca2+]i increased from 0.25 to 2 microM following both fertilization and activation and returned to the unactivated level after about 37 min. Immature oocytes of D. pictus were also studied with the vibrating probe and the inward current in these cells was much less localized than that in the activating egg. A steady transcellular current of up to 4 microA/cm2 entered the entire animal hemisphere of the oocyte and exited the vegetal hemisphere.     

Interfacial instability and membrane internalization in human erythrocytes heated in the presence of serum albumin

The dynamics of morphological change, when human erythrocytes are heated through the spectrin denaturation temperature in the presence of bovine serum albumin, has been studied using differential interference contrast optics and a television video analysis system. Most washed (control) cells developed a wavy disturbance, with an average of $\text{6.6 ± 0.4}$ (2 S.E.) waves per cell rim, when heated. The average number of waves per cell rim decreased and the percentage of heated cells showing morphological changes in the dimple region increased with increasing serum albumin concentration, reaching 100% at 1.0 g/l. The change in the dimple region of cells heated in the presence of serum albumin involved the growth of a regular wavy disturbance around the cell dimple rim. The development of the wavy disturbance on the dimple, which resulted in the internalization of membrane, has been examined as an example of an interfacial instability on a biological membrane. Scanning and transmission electron micrographs confirm membrane internalization.     

Fertilization in Discoglossus pictus (Anura). I. Sperm-egg interactions in distinct regions of the dimple and occurrence of a late stage of sperm penetration

The heterogeneity of the egg surface with respect to receptivity to sperm was investigated in Discoglossus pictus; in this species fertilization occurs only in an indentation called the dimple, at the center of the animal hemisphere. Following insemination sperm are seen in the outermost jelly layers and in the lens-shaped jelly plug, converging to the dimple center, D1. A fertilization potential (FP) is recorded 30 sec following insemination. About 30 min after fertilization, when fertilization cones can be detected easily, immotile sperm are found at the center of the cone, where 10 min later they accomplish penetration. After 15 min the cone regresses and the second polar body is extruded. In eggs where the plug was experimentally displaced with respect to the dimple, spermatozoa contacted the sides of the dimple and simple protrusions formed but not cones. Spermatozoa do not elicit a normal FP in these regions but small step depolarizations which may be followed by a gradual rise to a positive plateau potential. Such eggs do not develop. In the protrusions, sperm may be only partially incorporated and the unpenetrated portion appears to degenerate. We conclude that at least two regions exist in the dimple: D1, where the FP is triggered, cones are formed, sperm penetration is fully accomplished and development is initiated; and D2 + D3 where the electrical response is not a normal FP, cones do not form, total sperm penetration does not occur, and development is not initiated.     

Antispectrin antibodies stain the oocyte nucleus and the site of fertilization channels in the egg of Discoglossus pictus (Anura).

In Discoglossus pictus eggs, only the dimple contains ionic channels active at fertilization; in particular, chloride channels are found in the central portion of the dimple, which is also the site of sperm penetration. Moreover the dimple hosts an imposing cytoskeleton, consisting of a cortical network and bundles of microfilaments extending from the microvilli. Since spectrin cross links actin and is connected through ankyrin to anion transporters in the plasma membrane of erythrocytes as well as to anion channels in other cells, we studied, in D. pictus egg, the relationship between the localization of spectrin and the high polarization of ionic channels and cytoskeletal organization. By means of immunocytochemistry, we localized spectrin exclusively in the egg dimple. In an attempt to trace back the source of spectrin localization, we immunostained sections of D. pictus ovary and localized spectrin in the nuclei of previtellogenic oocytes, where actin is also present. Antispectrin staining remained until germinal vesicle breakdown. By contrast, a cortical localization was found only when the oocytes divided into two hemispheres and into the germinative area (GA), which, after germinal vesicle breakdown, gives rise to the dimple. At this stage the antispectrin signal was particularly strong in the GA. Using Rho-pialloidin, we also established that spectrin is generally present where F-actin is found. However, spectrin and F-actin do not have the same pattern of fluorescence. In conclusion, our data suggest that spectrin may play a role in oocyte and egg polarity. In eggs, it could be instrumental in anchoring to the cytoskeleton membrane proteins such as receptors and ionic channels, including chloride-permeable channels.     

Lipovitellin constitutes the protein backbone of glycoproteins involved in sperm-egg interaction in the amphibian Discoglossus pictus

Our knowledge of the molecules that interact with sperm at the egg membrane is restricted to a short list. In the eggs of Discoglossus pictus, fusion with sperm is limited to a differentiated structure, the dimple, offering several advantages for detecting molecules involved in fertilization. Previous studies have identified fucosylated glycoproteins of 200, 260, and 270 kDa located at the surface of the dimple that are able to bind sperm in vitro. Here, we show that dimple glycoproteins and a protein represented by a 120‐kDa band released following gel‐into‐gel SDS–PAGE of both glycoproteins share the same N‐terminal amino acid sequence, which itself is similar to the N‐termini of Xenopus liver‐synthesized vitellogenin (VTG) and the lipovitellin 1. MALDI/MS mass spectrometry indicated that the 120‐kDa band is part of both gps 200 and 270/260. A 117‐kDa major protein of the egg lysate exhibits the same MALDI/MS spectrum, and LC‐MSMS indicates that this is a lipovitellin 1 (DpLIV) that coincides with the 120‐kDa band and is responsible for the formation of the 200–270‐kDa dimers. Therefore, lipovitellin 1 constitutes the protein backbone of the dimple glycoconjugates. In vitro assays using polystyrene beads coated with DpLIV or with its dimers indicate that significant sperm binding occurs only with DpLIV dimers. In amphibians, VTG is taken up by the oocyte, where it releases lipovitellins destined to form yolk. In Discoglossus, our data suggest that yolk proteins are also synthesized by the oocyte. The dimple forms in the ovulated oocyte following the exocytosis of vesicles that likely expose DpLIVs at their membrane. Indeed, in whole mounts of immunostained eggs, anti‐vitellogenin antibodies label only the surface of the dimple. Mol. Reprod. Dev. 78:161–171, 2011. © 2011 Wiley‐Liss, Inc.     

Evidence from studies of birefringence of structure across the dimple region of red cells

Analysis of the equilibrium of the normal biconcave human red cell, in terms of its tension and a pressure inside, suggests a force of attraction between the opposite membranes at the dimple regions. The analogous attraction that causes rouleaux formation is mediated by long-chain molecules. Single cells hanging on edge between polarizer and analyser, almost “crossed,” were photographed at different angles to the axis of the polarizer. Enlarged prints were scanned by a photometer. For single cells the records showed non-significant fluctuations of intensity, but mean values for 32 cells showed a very significant sinusoidal variation with angle, as predicted by theory for birefringence in the cell at the dimple region. For the rim region, the averaged data showed no variation with angle. In cells moderately osmotically swollen, birefringence in the centre of the dimple region was absent, but persisted close to the inside of the membranes. The latter disappeared in cells further swollen to a biconvex shape. The data is interpreted as indicating oriented chains of molecules across the interior of the cell at the dimple region. The behaviour on swelling was what had been seen in a model with nylon fibres oriented between the charged plates of a condenser, in which the variation of attractive force with distance was adequate to explain the equilibrium of the red cell membrane.     

Navigation in Marine Protected Areas: National and International Law

Abstract

World fish resources, fishing methods, and processing operations in the seafood industry are described. The fishery situation in developing countries (LDCs) is discussed, with particular reference to artisanal and other local fisheries, and examples are cited to illustrate the structure of the industry. Technology transfer from developed countries to LDCs is discussed and recommendations are presented for future technology transfer programs. It is concluded that an integrated complex of small projects with defined, attainable objectives and immediate impact on income and food supply of the LDC populations is likely to be more successful than large‐scale programs with little immediate payoff. A case study of fisheries in two developing countries, Thailand and Peru, and extensive tabulation of statistical data on catches, value of catch, and unit value of fish species groups for selected countries, with a discussion of the significance of the data, are presented in an appendix.     

The cortical reaction in the egg of Discoglossus pictus: a study of the changes in the endoplasmic reticulum at activation

In Discoglossus pictus previous ultrastructural observations have shown that at the animal dimple, where sperm fuse with the egg, cortical granules (CG), vacuoles, and tightly packed clusters of small cisternae are present. At fertilization the clusters open (i.e., become loose) and give rise to longer cisternae arranged in whorls and chains which migrate toward the plasma membrane. The vacuoles fuse to form cisternae and exocytose along with the CG. In the rest of the egg periphery, while exocytosis occurs, the clusters do not open as a result of activation (C. Campanella, R. Talevi, U. Atripaldi, and L. Quaglia (1986). In "Molecular and Cellular Biology of Fertilization" (J.L. Hedrick, Ed.). Plenum, New York). We have recently conducted electrophysiological studies which have detected inward currents at the dimple center, outward current at the rest of the egg surface, and an eightfold increase in [Ca2+]i which propagates from the site of activation throughout the egg (R. Nuccitelli, D. Kline, W. Busa, R. Talevi, and C. Campanella (1988). Dev. Biol. 130, 120-132). In this paper we have asked whether the anionic current and the Ca2+ increase could be causally related to the changes of the smooth endoplasmic reticulum (SER) at activation. The results obtained by activating the eggs in ion-substituted Ringers indicate that (1) the migration of cisternae is not dependent on the polarity of the activation current crossing the dimple, but is strongly impaired, together with CG exocytosis, by 5 x Cl- Ringer; (2) TMB-8, a drug which partially blocks calcium release (C. Y. Choiu and M. J. Malagodi (1975). Brit. J. Pharmacol. 53, 279-288), partially inhibits opening of cisternae clusters and the formation of an SER network in the dimple. This suggests a causal relationship between the Ca2+ rise and the cluster transformation at activation.