基于生态系统评价的山水林田湖草生态保护与修复体系构建研究——以乌梁素海流域为例

山水林田湖草系统保护与修复工程实施的重要目标是维护和提升区域生态系统服务。从乌梁素海流域山水林田湖草的生态现状与功能出发,对乌梁素海流域水土流失、土地沙化等生态敏感性及土壤保持、水源涵养、生物多样性等生态功能重要性进行系统评价,形成基于生态敏感性和生态功能重要性相结合的空间格局评价结果。以维护和提升人类福祉所需的重要生态系统服务为目标,以乌梁素海流域生态敏感性和生态功能重要性相结合的空间格局评价结果为基础,制定了“一中心、二重点、六要素、七工程”的乌梁素海山水林田湖草生态保护与修复体系,并基于此将乌梁素海流域生态保护修复分为6个主要治理区域,形成“四区、一带、一网”的生态安全格局,通过具体工程实施,流域生态环境质量和生态服务能力将取得明显提升,防风固沙能力有效增强,生物多样性持续改善,水环境质量稳定达标,生态系统的稳定性明显加强。通过乌梁素海流域的分析案例为流域山水林田湖草生态保护与修复关键区域的识别提供了定量分析方法,为流域尺度构建生态安全格局、实现山水林田湖草系统保护和修复提供思路和途径。     

胞间连丝与大分子物质的胞间转运机制

胞间连丝是相邻细胞间共质体运输的桥梁。基于对胞间连丝分子组成及超微结构的研究,不同学者提出了不同的胞间连丝结构模型。对其功能的研究表明,胞间连丝在物质运输、信息传递、病毒的周身感染等方面都具有重要作用。文章就胞间连丝的结构、分子组成及病毒介导的大分子胞间转移,以及对内源蛋白质的胞间转运机制诸方面的研究进展作了概述。     

生物素标记钙调素用于植物钙调素结合蛋白的检测

用生物素标了己了花椰菜ＣａＭ。生物素标记的ＣａＭ具有与天然ＣａＭ相似的Ｃａ２＋依赖电泳特性,可激活ＣａＭ依赖性磷酸二酯酶,能够检测出５０ｎｇ的磷酸二酯酶。利用它建立了检测植物ＣａＭ结合蛋白的生物素－覆盖法（Ｂｉｏｔｉｎ－ｏｖｅｒｌａｙ）并证实酶标亲和素可与胡萝卜愈伤组织内６４ｋＤ蛋白质非特异结合,因此将此法运用于植物材料时必需设置酶标亲和素处理的对照。用生物素－覆盖法检测胡萝卜愈伤组织形成过程中的ＣａＭ结合蛋白时可检出２,４－Ｄ诱导的ＣａＭ结合蛋白。     

HCMV大小鼠眼组织损伤模型的初步研究

目的探讨接种人巨细胞病毒(Humancytomegalovirus,HCMV)是否引起Wistar大鼠、昆明种小鼠眼组织损伤.方法将HCMVAD169毒株经静脉接种Wistar大鼠和昆明种小鼠,观察动物眼部发病情况,原位杂交检测动物眼组织中的HCMVDNA片段.结果接种病毒后部分动物缓慢出现眼部发病,局部分泌物增多、浑浊甚至失明;经原位杂交于视锥、视杆细胞和角膜内皮细胞中检出HCMVDNA片段.结论HCMV可以感染动物眼组织,并引起动物发生眼病.     

植物基因表达的代谢调控

通过分析代谢物、激素和环境因素对植物几种基因表达的影响,就植物基因表达的代谢调控进行了讨论,提出了开展有关这方面研究的一些设想。     

接种外生菌根对辽东栎幼苗生长的影响

 辽东栎（Quercus liaotungensis）是中国特有的栎林树种,也是中国暖温带落叶阔叶林的主要优势树种之一。铆钉菇（Gomphidius viscidus）和臭红菇（Russula foetens）是在自然环境中与其共生形成外生菌根的真菌。在温室花盆中播种辽东栎种子获得辽东栎幼苗,并对幼苗接种铆钉菇和臭红菇合成外生菌根,比较了有菌根和无菌根辽东栎幼苗生长、光合蒸腾特性、氮磷含量的差异。外生菌根对辽东栎幼苗的生长有明显的促进作用,有菌根幼苗的生物量、株高、净光合速率和水分利用效率高于无菌根幼苗,蒸腾速率则相反。有菌根幼苗的氮磷含量分别为无菌根幼苗的1.7倍和2.2倍,外生菌根的合成还改变了氮磷在幼苗器官间的分配比例,与无菌根幼苗相比,有菌根幼苗茎中的氮磷减少,而叶片中的磷显著增加。同时接种铆钉菇和臭红菇的生长促进效果优于单独接种。     

拟南芥PKA催化亚基基因的克隆、原核表达及其催化活性的鉴定

蛋白质的磷酸化与脱磷酸化是生物体内存在的一种普遍的调节方式，几乎参与所有的生命活动过程。利用Blast2.0分析拟南芥基因组序列发现存在一个与动物蛋白激酶cDNA同源性的序列。在GenBank中比较发现它与动物的依赖cAMP的蛋白激酶（PKA）的催化亚基（C亚基）有相似的特征序列。提取拟南芥（Arabidopsis thaliana (L.)Heynh.)的总ＲＮＡ，通过ＲＴ－ＰＣＲ克隆得到这一cDNA片段，经序列测定证实它具有完整的阅读框架，将其克隆至pET30a原核表达载体，结果表明在大肠杆菌（E.coli)BL21(DE3)中该表达质粒在IPTG诱导下表达产生大量带寡聚组氨酸标记的重组蛋白，该蛋白在37℃表达时主要以包含体形式存在，而在22℃表达时主要以可溶性蛋白形式存在，经过与组氨酸结合金属螯合树脂亲和柱层析纯化后，得到纯化的目的蛋白，其纯度达到87%以上。活性鉴定表明其具有依赖于cAMP的蛋白激酶活性。而加入PKA的抑制剂（H-8）后，其活性显著下降。从而证实它确实是拟南芥的PKA催化亚基。Western blot结果显示它几乎不受ABA，NaCl等逆境的诱导。     

Using a modified TA cloning method to create entry clones

We describe a noncommercial alternative method to create entry clones compatible with all kinds of destination vectors based on an improved TA cloning approach. To generate Gateway T vectors, we first constructed gentamicin- and chloramphenicol-resistant entry vectors designated pGWG and pGWC, respectively. Each entry vector contains an AhdI cassette flanked by attL sites, with each AhdI cassette containing two AhdI restriction enzyme sites spaced by the ccdB killer gene, which is lethal to most Escherichia coli strains. Gateway T vectors can be prepared by simple digestion of these entry vectors with the AhdI enzyme or its isoschizomers. The use of the ccdB gene as a negative selection marker is an important improvement over conventional TA cloning in that it eliminates the necessity of blue/white color screening based on alpha-complementation. Another important improvement that we have implemented is to retail the T vectors using Taq polymerase and dTTP so as to improve the cloning efficiency. Together, these improvements allow TA cloning to realize its full potential. Using Gateway T vectors prepared by this improved method, entry clones for PCR products or restriction enzyme fragments can be created simply, efficiently, and inexpensively while at the same time introducing greater compatibility.     

A Signaling Pathway Linking Nitric Oxide Production to Heterotrimeric G Protein and Hydrogen Peroxide Regulates Extracellular Calmodulin Induction of Stomatal Closure in Arabidopsis

Extracellular calmodulin (ExtCaM) regulates stomatal movement by eliciting a cascade of intracellular signaling events including heterotrimeric G protein, hydrogen peroxide (H₂O₂), and Ca²⁺. However, the ExtCaM-mediated guard cell signaling pathway remains poorly understood. In this report, we show that Arabidopsis (Arabidopsis thaliana) NITRIC OXIDE ASSOCIATED1 (AtNOA1)-dependent nitric oxide (NO) accumulation plays a crucial role in ExtCaM-induced stomatal closure. ExtCaM triggered a significant increase in NO levels associated with stomatal closure in the wild type, but both effects were abolished in the Atnoa1 mutant. Furthermore, we found that ExtCaM-mediated NO generation is regulated by GPA1, the Gα-subunit of heterotrimeric G protein. The ExtCaM-dependent NO accumulation was nullified in gpa1 knockout mutants but enhanced by overexpression of a constitutively active form of GPA1 (cGα). In addition, cGα Atnoa1 and gpa1-2 Atnoa1 double mutants exhibited a similar response as did Atnoa1. The defect in gpa1 was rescued by overexpression of AtNOA1. Finally, we demonstrated that G protein activation of NO production depends on H₂O₂. Reduced H₂O₂ levels in guard cells blocked the stomatal response of cGα lines, whereas exogenously applied H₂O₂ rescued the defect in ExtCaM-mediated stomatal closure in gpa1 mutants. Moreover, the atrbohD/F mutant, which lacks the NADPH oxidase activity in guard cells, had impaired NO generation in response to ExtCaM, and H₂O₂-induced stomatal closure and NO accumulation were greatly impaired in Atnoa1. These findings have established a signaling pathway leading to ExtCaM-induced stomatal closure, which involves GPA1-dependent activation of H₂O₂ production and subsequent AtNOA1-dependent NO accumulation.Plant guard cells control opening and closure of the stomata in response to phytohormones (e.g. abscisic acid [ABA]) and various environmental signals such as light and temperature, thereby regulating gas exchange for photosynthesis and water status via transpiration (Schroeder et al., 2001). Cytosolic calcium ([Ca²⁺]_i) has been shown to be a key second messenger that changes in response to multiple stimuli in guard cells (McAinsh et al., 1995; Grabov and Blatt, 1998; Wood et al., 2000). A large proportion of Ca²⁺ is localized in extracellular space. It has been shown that external Ca²⁺ concentration ([Ca²⁺]_o) promotes stomatal closure and induces oscillation in [Ca²⁺]_i in guard cells (MacRobbie, 1992; McAinsh et al., 1995; Allen et al., 2001). However, how the guard cells perceive [Ca²⁺]_o concentration and convert [Ca²⁺]_o changes into [Ca²⁺]_i changes was not understood until a calcium-sensing receptor (CAS) in the plasma membrane of guard cells in Arabidopsis (Arabidopsis thaliana) was identified (Han et al., 2003). The external Ca²⁺ (Ca²⁺_o)-induced [Ca²⁺]_i increase is abolished in CAS antisense lines (Han et al., 2003). Both [Ca²⁺]_o and [Ca²⁺]_i show diurnal oscillation that is determined by stomatal conductance, whereas the amplitude of [Ca²⁺]_i oscillation is reduced in CAS antisense lines (Tang et al., 2007). The reduced amplitude of [Ca²⁺]_i diurnal oscillation in response to Ca²⁺_o treatment suggests the potential existence of other [Ca²⁺]_o sensor(s) that may transmit [Ca²⁺]_o information into the [Ca²⁺]_i response in coordination with CAS. Extracellular calmodulin (ExtCaM) could be such an additional [Ca²⁺]_o sensor.Calmodulin is a well-known Ca²⁺ sensor that is activated upon binding of Ca²⁺. It has been shown that calmodulin exists not only intracellularly but also extracellularly in many plant species (Biro et al., 1984; Sun et al., 1994, 1995; Cui et al., 2005). ExtCaM has been implicated in several important biological functions, such as the promotion of cell proliferation, pollen germination, and tube growth (Sun et al., 1994, 1995; Ma and Sun, 1997; Ma et al., 1999; Cui et al., 2005; Shang et al., 2005). ExtCaM is found in the cell wall of guard cells in Vicia faba and in the epidermis of Arabidopsis by immunogold labeling/electron microscopy and western-blot analyses, respectively, and the endogenous CaM in the extracellular space has been shown to regulate stomatal movements (Chen et al., 2003; Xiao et al., 2004). Under natural conditions, once the activity of ExtCaM has been inhibited by its membrane-impermeable antagonist W7-agrose or CaM antibody, stomatal opening under light is enhanced and stomatal closure in darkness is inhibited in V. faba and Arabidopsis (Chen et al., 2003; Xiao et al., 2004). [Ca²⁺]_i and cytosolic hydrogen peroxide (H₂O₂) changes, two events involved in ExtCaM-regulated stomatal movement (Chen et al., 2004), are likely regulated by light/darkness (Chen and Gallie, 2004; Tang et al., 2007), suggesting that ExtCaM plays an important physiological role in the regulation of stomatal diurnal rhythm. Calmodulin-binding proteins have been found in the protoplast of suspension-cultured Arabidopsis cells, supporting the idea that ExtCaM functions as a peptide-signaling molecule (Cui et al., 2005). Furthermore, ExtCaM triggers [Ca²⁺]_i elevation in guard cells of V. faba and Arabidopsis and in lily (Lilium daviddi) pollen (Chen et al., 2004; Xiao et al., 2004; Shang et al., 2005). These observations support the notion that ExtCaM could be a potential [Ca²⁺]_o sensor for external calcium, and this external calcium sensing could subsequently regulate the [Ca²⁺]_i level through a signaling cascade.It is interesting that ExtCaM and ABA induce some parallel changes in second messengers in guard cell signaling. Our previous studies show that ExtCaM induces [Ca²⁺]_i increase and H₂O₂ generation through the Gα-subunit (GPA1) of a heterotrimeric G protein, and increased H₂O₂ further elevates [Ca²⁺]_i (Chen et al., 2004). G protein, Ca²⁺, and H₂O₂ are well-known second messengers in ABA-induced guard cell signaling (McAinsh et al., 1995; Grabov and Blatt, 1998; Pei et al., 2000; Wang et al., 2001; Zhang et al., 2001; Liu et al., 2007). However, the signaling cascade triggered by ExtCaM in guard cells is poorly understood. New ABA signaling components in guard cells could provide a clue in the study of the molecular mechanism of ExtCaM guard cell signaling.Recently, nitric oxide (NO) has been shown to serve as an important signal molecule involved in many aspects of developmental processes, including floral transition, root growth, root gravitropism, adventitious root formation, xylogenesis, seed germination, and orientation of pollen tube growth (Beligni and Lamattina, 2000; Pagnussat et al., 2002; He et al., 2004; Prado et al., 2004; Gabaldón et al., 2005; Stohr and Stremlau, 2006). Increasing evidence points to a role for NO as an essential component in ABA signaling in guard cells (Garcia-Mata and Lamattina, 2001, 2002; Neill et al., 2002). It has been shown that nitrate reductase (NR) reduces nitrite to NO, and the nia1, nia2 NR-deficient mutant in Arabidopsis showed reduced ABA induction of stomatal closure (Desikan et al., 2002; Bright et al., 2006). Although animal nitric oxide synthase (NOS) activity has been detected in plants and inhibitors of mammalian NOS impair NO production in plants (Barroso et al., 1999; Corpas et al., 2001), the gene(s) encoding NOS in plants is still not clear. AtNOS1 in Arabidopsis was initially reported to encode a protein containing NOS activity (Guo et al., 2003). However, recent studies have raised critical questions regarding the nature of AtNOS1 and suggested that AtNOS1 appears not to encode a NOS (Crawford et al., 2006; Zemojtel et al., 2006). However, the originally described Atnos1 mutant is deficient in NO accumulation (Crawford et al., 2006). Consequently, AtNOS1 was renamed AtNOA1 (for NITRIC OXIDE ASSOCIATED1; Crawford et al., 2006). Therefore, the Atnoa1 mutant provides a useful tool for dissecting the function of NO in plants. At present, the molecules that regulate NO generation in ABA-mediated guard cell signaling are not clear. Evidence suggests that H₂O₂, a second messenger important for the regulation of many developmental processes and stomatal movement (Pei et al., 2000; Zhang et al., 2001; Coelho et al., 2002; Demidchik et al., 2003; Kwak et al., 2003), regulates NO generation in guard cells (Lum et al., 2002; He et al., 2005; Bright et al., 2006).Given the parallel signaling events induced by ABA and ExtCaM, we investigated whether NO is involved in the regulation of ExtCaM-induced stomatal closure in Arabidopsis and whether it is linked to G protein and H₂O₂, two key regulators of both ExtCaM and ABA regulation of stomatal movements. Using Arabidopsis mutants (e.g. GPA1 null mutants, the NO-producing mutant Atnoa1, and the guard cell H₂O₂ synthetic enzymatic mutant atrbohD/F) combined with pharmacological analysis, we present compelling evidence to establish a linear functional relationship between Gα, H₂O₂, and NO in ExtCaM guard cell signaling.