民勤荒漠区植物物候型特征及其与气温的关系

对民勤荒漠区34年的物候观测资料进行了物候型分析。结果表明：植物的萌动期有2种物候型,展叶期和开花期各有4种物候型,果熟期有2种物候型,1974年以来,当地年平均气温和2、3、6月月平均气温有较显著的增温趋势,与此同时,植物的春季物候期亦有明显的提前趋势,低温-短日照-早萌动物候型的芽膨大期34年提前了9.7 d;从萌动期→展叶期→开花期→果熟期,物候期的提前幅度逐渐减小;物候期提前主要与当月气温升高有关;萌动期2种物候型和展叶期4种物候型是植物对春季气温和秋末冬初气温适应性的分异,开花期4种物候型和果熟期2种物候型是植物花期多样性和果熟期多样性对当地干旱环境适应性的反应。     

开放式空气C02浓度增高对水稻冠层能量平衡的影响

大气CO2浓度升高对植物冠层能量平衡的影响是导致植物生长发育和水分利用率发生变化的环境物理原因．利用位于江苏省无锡市安镇的农田自由开放式空气CO2浓度增高(FACE)系统平台,进行水稻冠层微气候和土壤热通量的连续观测,并结合能量平衡分析,研究了FACE对水稻冠层能量平衡的影响．结果表明,水稻冠层显热和潜热通量FACE与对照的差异日最大值出现在14：00左右,与空气相对湿度日最低值出现时间一致;潜热通量FACE与对照的差异日最大值变化在—15-—65J·m^-2·s^-1之间,显热通量FACE与对照的差异最低值变化在12—55J·m^-2·s^-1之间;显热和潜热通量FACE与对照的差异日最大值随冠层上方辐射平衡增加而增大．水稻冠层白天总显热通量FACE均高于对照,而总潜热通量FACE均低于对照．白天总显热和潜热通量FACE与对照的差异在同一生育期内随冠层上方净辐射增强而增大,在不同生育期随生育期推进而减少．开花期至蜡熟期,水稻冠层白天总潜热通量FACE比对照平均低6．7％．FACE使水稻冠层白天总显热通量及其占冠层上方辐射平衡的比例减少,而使总潜热通量及其占冠层上方辐射平衡的比例增大,但对土壤热通量及夜间显热和潜热通量的影响不大．开花期至蜡熟期水稻冠层白天总显热、潜热通量占冠层上方净辐射总量的比例FACE与对照之差平均为5．5％．     

盐生荒漠地表水热与二氧化碳通量的季节变化及驱动因素

以古尔班通古特沙漠南缘原始盐生荒漠为对象,利用涡度相关法,对原始盐生荒漠地表水热、二氧化碳通量进行了连续观测,对通量的季节变化、浅层土壤水分条件改变对盐生荒漠植物群落水汽、二氧化碳通量以及水分利用效率的影响进行了系统的分析.结果表明:净辐射通量、潜热通量和二氧化碳通量都具有明显的季节变化趋势,而显热通量的季节变化不明显.在有效能量的分配上,显热通量是有效能量的主要输出项.在降水影响期和非影响期,二氧化碳通量没有明显的变化;而在非降水影响期潜热通量明显降低,表明土壤水分处于亏缺状态,但二氧化碳通量并没有降低的趋势,而与前期保持高度的一致性.以此可以推断,该荒漠盐生植物群落并不以降水为主要水分来源,降水后水汽通量和二氧化碳通量变化的不一致性是该原始盐生荒漠独特植物特征决定的.降水影响期原始盐生荒漠植物群落的水分利用效率低于非影响期,是由于降水后土壤蒸发迅速增加,而植物蒸腾与光合并未随之增加造成的.     

季节性干旱对中亚热带人工林显热和潜热通量日变化的影响

植被与大气间的显热和潜热通量的日变化是大气过程和植被生理过程的显著标志。本研究利用ChinaFLUX千烟洲站典型的夏季雨热不同季的季节性干旱的试验条件,探讨了2003年季节性干旱对该生态系统显热和潜热通量日变化变异幅度和峰值时间的影响。研究表明：显热通量的日变化变异幅度年平均值为176 W/m2。潜热通量的日变化变异幅度年平均值为171 W/m2。显热通量到达日变化峰值的时间平均为11:57。全年潜热通量的日变化都在午后达到峰值,平均值为12:33。季节性干旱造成显热通量的日变异幅度明显增大,从144W m-2增加到321 W m-2。而潜热通量的日变异幅度明显降低,从324 W/m2减小到198 W/m2。,显热和潜热通量日变异幅度的相对变化明显增大,从-165 W/m2增加到76 W/m2,气温和饱和水汽压差是影响显热和显热日变异幅度及其相对变化的主要控制因素。干旱胁迫期,深层水对显热通量日变化变异幅度及其与潜热通量日变化变异幅度的相对变化的作用更显著,而潜热通量日变化变异幅度与气象要素关系不显著。季节性干旱造成显热通量日变化的峰值时间和显热和潜热通量日变化峰值时间的相对变化明显向下午偏移,显热通量日变化的峰值从上午11:31到中午12:17,相对变化从1小时到1小时20分钟。季节性干旱对潜热通量日变化峰值时间没有显著的影响。非干旱胁迫期,显热通量日变化峰值时间和显热及潜热通量日变化峰值时间的相对变化均与气温负相关,而干旱胁迫期,则与气温正相关。潜热通量日变化峰值时间与气象要素关系均不显著。该生态系统显热和潜热通量日变化峰值的相对变化主要受降水量的季节分配控制,在干旱胁迫期降水的作用更加明显。潜热和显热通量日变化峰值时间的相对变化总体上都受植被与大气间的耦合程度控制。     

亚热带毛竹林生态系统能量通量及平衡分析

利用开路涡度相关系统和常规气象观测仪器,对亚热带(浙江省)毛竹林生态系统2011年的净辐射、显热通量、潜热通量、土壤热通量以及气温、地温、降雨量等气象要素进行了连续观测,定量分析了毛竹林生态系统能量通量的变化和各能量分量的分配特征,并计算了能量闭合度以及波文比。结果表明:毛竹林全年净辐射为2628.00 MJ/m2,显热通量为576.80 MJ/m2,潜热通量为1666.77 MJ/m2,土壤热通量为-7.52 MJ/m2,土壤为热源,各能量分量季节变化明显,日变化基本呈单峰型曲线变化。显热通量占净辐射的22.0%,潜热通量占63.4%,毛竹林生态系统潜热通量为能量散失的主要形式。波文比逐月变化规律不明显,波动较大,在0.07—1.77之间变化,能量平衡比率法得出毛竹林年能量闭合度为0.85,月平均闭合度为0.84,能量闭合度高于线性回归法计算结果,但仍有15%的能量不闭合。     

高效经营雷竹林生态系统能量通量过程及闭合度

利用开路涡度相关系统和常规气象仪,对高效经营的雷竹林生态系统2011年的显热通量、潜热通量、净辐射、土壤热通量以及气温、地温、降雨量进行了观测,分析该生态系统能量通量的变化,以及各能量分量的分配特征,并计算了波文比及能量闭合.结果表明：雷竹林全年净辐射为2928.92 MJ·m^-2,潜热通量、显热通量和土壤热通量分别为1384.90、92754和-28.27 MJ·m^-2,各能量分量的日变化和月变化基本呈单峰曲线.潜热通量为能量散失主要形式,占净辐射的47.3%,显热通量占31.7%,波文比呈“U”型曲线,在0.285～2.062之间变化,土壤为热源.雷竹林年能量闭合度为0.782,月平均闭合度为0.808.
     

我国亚热带毛竹林生长季能量通量过程及闭合度分析

为探讨我国亚热带毛竹林(Phyllostachys edulis)生长季的能量平衡关系,利用开路涡度相关法,对2011年毛竹林生长季的能量通量的变化特征进行了研究,并应用能量平衡比率法和线性回归2种方法,分析了能量闭合的特点。结果表明,我国亚热带毛竹林生长季的净辐射总量为1738.2 MJ m–2,显热通量为354.3 MJ m–2,潜热通量为1146.0 MJ m–2,土壤热通量为58.9 MJ m–2,土壤为热汇,显热通量占净辐射的20.4%,潜热通量占65.9%,土壤热通量占3.4%。毛竹林生长季的能量闭合度为0.89,月平均闭合度为0.91,但仍有11%的能量不闭合。可见,毛竹林生长季以潜热能量散失形式为主,各能量分量均以净辐射变化为基础,且日变化基本呈单峰型曲线。     

长白山阔叶红松林生长季热量平衡变化特征

根据长白山阔叶红松林2001年5月下旬至10月上旬微气象梯度观测资料和辐射、土壤热通量资料,用波文比-能量平衡方法(BREB方法)计算了森林的显热通量和感热通量,并计算了森林大气和植被体的储热量,分析了阔叶红松林热量平衡各项的日变化和季节变化,结果发现,热量平衡(净辐射)与太阳总辐射呈线性关系;热量平衡各项都与净辐射有相同的日变化特征,为昼正夜负的曲线．各项的绝对值一般表现为净辐射>潜热通量>感热通量>储热变化．受日照时间的影响,6～10月各分量正值的日持续时间逐渐缩短．月平均结果,白天净辐射6月份最大,10月上旬最小,变化于0～527W·m^-2,夜间的净辐射在0～-121W·m^-2．潜热通量白天和夜间分别在0～441、0～-81W·m^-2,感热通量昼夜分别在0～80、0～-26W·m^-2．储热变化则为0～44、0～-26W·m^-2．白天潜热通量占净辐射的比例8～10月逐渐下降,而感热通量和储热变化的比例9～10月明显上升,特别在严霜后2～3d,出现潜热通量比例突减、感热通量比例突增的现象．文中还对通量观测仪器、方法进行了简要分析．     

华北人工林水热碳通量环境影响因子分析

基于河北崇陵流域人工林涡度相关通量观测数据,采用通径分析和分段回归解析了水热碳通量与土壤水分、饱和水汽压差、空气和土壤温度,及净辐射、光合有效辐射等环境因子的关联性。结果表明,通径分析法揭示了各指标的主导/次要因子的直接及间接效应,显热通量和水分利用效率的主要影响因子为饱和水汽压差,而潜热通量、碳通量的影响因子以辐射、温度为主;分段回归法进一步探讨了次要因子对主导因子的限制作用,当0.20 m3·m–3土壤水分含量≤0.35 m3·m–3时,潜热通量、生态系统呼吸及水分利用效率与其主导因子间相关性最高,当饱和水汽压差≤1.0 k Pa时,净生态系统生产力、总生态系统生产力与其主导因子间相关性最高;两种方法的有机结合,使我们对生态水文过程各驱动因子有了清晰的宏观认识,并量化了次要因子起限制作用的数量范围。     

黄土高原农牧交错带稀疏自然植被生态系统的地表能量特征

基于2011-2012年黄土高原农牧交错带稀疏自然植被生态系统的地表能量通量以及气象数据,对该地区能量平衡各分量(净辐射、感热、潜热和土壤热通量)以及波文比进行日、季节动态的特征分析,研究了潜热通量和感热通量对不同强度降雨事件响应程度的差异,并分析了潜热通量和感热通量的主控因子.结果表明:该地区净辐射、感热、潜热和土壤热通量的日、季节动态曲线均为单峰型曲线,净辐射、感热通量、潜热通量和土壤热通量的年平均值分别为78.19、33.32、24.91和2.65 W·m-2.在全年能量收支平衡中,感热通量占净辐射的43％,潜热通量占32％,土壤热通量占3％,表明对于黄土高原农牧交错带自然稀疏灌木生态系统,全年能量主要以感热的形式交换.生长季感热和潜热占净辐射的比例相同(36％);而在非生长季,感热占主导,占净辐射的比例高达54％.潜热通量在强、弱降雨事件发生后明显升高,感热通量则明显下降.潜热通量与净辐射、水汽压差及植被参数均显著相关,感热通量与净辐射及空气温度梯度显著相关.     

黄花棘豆脱水素OoY_2K_4的鉴定及表达分析

该研究以黄花棘豆cDNA为模板,采用同源克隆法,从黄花棘豆转录组数据库中克隆获得1个响应逆境胁迫的胚胎发育晚期丰富蛋白基因,命名为OoY_2K_4;OoY_2K_4基因ORF为786bp,编码261个氨基酸,含有2个保守的Y片段和4个K片段,为典型的Y_2K_4类脱水蛋白亚家族成员;OoY_2K_4蛋白不具有跨膜结构域,不存在信号肽,亲水性极强,含有1个糖基化位点和17个磷酸化位点;亚细胞定位显示,OoY_2K_4蛋白定位于细胞质中。多序列比对发现,OoY_2K_4蛋白与其他物种第二组LEA蛋白(脱水素)序列高度保守;进化树分析显示,该序列与三叶草、蒺藜苜蓿和紫花苜蓿相似度最高,亲缘关系最近。采用qRT-PCR对OoY_2K_4基因在干旱、高盐、低温以及脱落酸、乙烯、赤霉素处理下的表达分析显示,干旱和高盐胁迫可显著诱导OoY_2K_4基因表达,而低温胁迫下基本无变化;激素处理均可诱导OoY_2K_4基因高效表达,其中脱落酸诱导下OoY_2K_4基因表达最显著。研究推测,OoY_2K_4基因可能通过依赖ABA的信号途径参与黄花棘豆对干旱和高盐逆境胁迫的应答反应。     

Na_2SeO_4对蛹虫草子实体生长的影响

蛹虫草是一种药食两用真菌,具有与冬虫夏草相似的功能,且富硒能力较强。本研究通过大量的人工栽培试验,旨在探究不同浓度Na_2SeO_4对新疆本地蛹虫草子实体生长的影响。试验表明,质量浓度为20 mg/L的Na_2SeO_4对蛹虫草的生长不产生显著影响,但蛹虫草各项生物学指标均随着培养基中外源Na_2SeO_4浓度的增加而呈下降趋势,说明随着外源Na_2SeO_4浓度的增加会对蛹虫草的生长产生抑制效应,当外源Na_2SeO_4质量浓度达到200 mg/L时,生产的蛹虫草已不具备商品价值。由此可见,20 mg/L的质量浓度是以Na_2SeO_4为硒源进行蛹虫草富硒研究的安全浓度。该研究为富硒产品开发寻找新的硒源开辟了新思路,为新疆地区进一步大规模栽培富硒蛹虫草提供一定的参考,但是对以Na_2SeO_4为硒源的最佳富硒浓度还有待于进一步研究。     

Nuclear genes required for post-translational steps in the biogenesis of the chloroplast cytochrome b6f complex in maize

Nuclear genes essential for the biogenesis of the chloroplast cytochrome b ₆ f complex were identified by mutations that cause the specific loss of the complex. We describe four transposon-induced maize mutants that lack cytochrome b ₆ f proteins but contain normal levels of other photosynthetic complexes. The four mutations define two nuclear genes. To identify the step at which each mutation blocks protein accumulation, mRNAs encoding each subunit were examined by Northern hybridization analysis and the rates of subunit synthesis were examined in pulse-labeling experiments. In each mutant the mRNAs encoding the known subunits of the complex were normal in size and abundance and the major subunits were synthesized at normal rates. Thus, these mutations block the biogenesis of the cytochrome b ₆ f complex at a post-translational step. The two nuclear genes identified by these mutations may encode previously unknown subunits, be involved in prosthetic group synthesis or attachment, or facilitate assembly of the complex. These mutations were also used to provide evidence for the authenticity of a proposed fifth subunit of the complex and to demonstrate a role for the cytochrome b ₆ f complex in protecting photosystem 11 from light-induced degradation.     

Modulation of the reductive metabolism of halothane by microsomal cytochrome b5 in rat liver

To study the modulation of the reductive metabolism of halothane (2-bromo-2-chloro-1,1,1-trifluoroethane) by microsomal cytochrome b₅, formation of 2-chloro-1,1,1-trifluoroethane (CTE) and 2-chloro-1,1-difluoroethylene (CDE), major reduced metabolites of halothane, was analyzed in vivo and in vitro. Rats were pretreated with both malotilate (diisopropyl-1,3-dithiol-2-ylidenemalonate) and sodium phenobarbital (malotilate-treated rats) or only with sodium phenobarbital (control rats). The microsomes of malotilate-treated rats had significantly more cytochrome b₅ than the controls, whereas the cytochrome P-450 content was not different between the two groups. At the end of 2-h exposure to 1% halothane in 14% oxygen, the ratio of CDE to CTE in arterial blood was significantly higher in malotilate-treated rats than in the controls. Under anaerobic conditions, the formation of CDE and the ratio of CDE to CTE were significantly greater in microsomal preparations of malotilate-treated rats than those of the controls. In a reconstituted system containing cytochrome P-450_PB purified from rabbit liver, addition of cytochrome b₅ to the system enhanced the formation of CDE and increased the ratio of CDE to CTE. These results suggested that cytochrome b₅ enhances the formation ratio of CDE to CTE by stimulating the supply of a second electron to cytochrome P-450, which might reduce radical reactions in the reductive metabolism of halothane.     

Involvement of plastoquinone bound within the isolated cytochrome b6-f complex from chloroplasts in oxidant-induced reduction of cytochrome b6

(1) Oxidant-induced reduction of cytochrome b₆ is completely dependent on a reduced component within the isolated cytochrome b₆-f complex. This component can be reduced by dithionite or by NADH/N-methylphenazonium methosulfate. It is a 2H⁺/2e⁻ carrier with a midpoint potential of 100 mV at pH 7.0, which is very similar to the midpoint potential of the plastoquinone pool in chloroplasts. (2) Oxidant-induced reduction of cytochrome b₆ is stimulated by plastoquinol-1 as well as by plastoquinol-9. The midpoint potential of the transient reduction of cytochrome b₆, however, was not shifted by added plastoquinol. (3) Quinone analysis of the purified cytochrome b₆-f complex revealed about one plastoquinone per cytochrome f. The endogenous quinone is heterogeneous, a form more polar than plastoquinone-A, probably plastoquinone-C, dominating, This is different from the thylakoid membrane where plastoquinone-A is the main quinone. (4) The endogenous quinone can be extracted from the lyophilized cytochrome b₆-f complex by acetone, but not by hydrocarbon solvents. Oxidant-induced reduction of cytochrome b₆ was observed in the lyophilized and hexane-extracted complex, but was lost in the acetone-extracted complex. Reconstitution was achieved either with plastoquinol-1 or plastoquinol-9, suggesting that a plastoquinol molecule is involved in oxidant-induced reduction of cytochrome b₆.     

贡嘎山峨眉冷杉树干呼吸空间特征及其对温度的响应

采用红外线气体分析仪-土壤呼吸气室水平测定法(HOSC)原位监测了贡嘎山东坡峨眉冷杉(Abies fabri)树干CO_2释放速率(E_s),分析了树干E_s与树干温度(T_(stem))的关系。贡嘎山峨眉冷杉树干E_s和T_(stem)空间变化格局明显,不同测定高度树干温度为0.3m1.3m2.3m,以1.3m处E_s最大;不同方向E_s和T_(stem)均表现为南面北面。生长季和非生长季的峨眉冷杉E_s分别在0.51—0.99μmol m~(-2)s~(-1)和0.14—0.22μmol m~(-2)s~(-1)之间波动。峨眉冷杉树E_s变化趋势和T_(stem)一致,二者具有显著的指数函数关系(P0.01)。峨眉冷杉非生长季树干呼吸Q_(10)显著高于生长季(P0.01),其中生长季变幅在1.9—3.0之间,非生长季在4.6—6.8之间,暗示个体或群落水平树干CO_2释放通量的估算应充分考虑树干E_s空间特征和Q_(10)变化。     

Identification of the polypeptides in the cytochromeb 6/f complex from spinach chloroplasts with redox-center-carrying subunits

An improved procedure for the isolation of the cytochromeb ₆/f complex from spinach chloroplasts is reported. With this preparation up to tenfold higher plastoquinol-plastocyanin oxidoreductase activities were observed. Like the complex obtained by our previous procedure, the complex prepared by the modified way consisted of five polypeptides with apparent molecular masses of 34, 33, 23, 20, and 17 kD, which we call Ia, Ib, II, III, and IV, respectively. In addition, one to three small components with molecular masses below 6 kD were now found to be present. These polypeptides can be extracted with acidic acetone. Cytochromef, cytochromeb ₆, and the Rieske Fe-S protein could be purified from the isolated complex and were shown to be represented by subunits Ia + Ib, II, and III, respectively. The heterogeneity of cytochromef is not understood at present. Estimations of the stoichiometry derived from relative staining intensities with Coomassie blue and amido black gave 1:1:1:1 for the subunits Ia + Ib/II/III/IV, which is interesting in of the presence of two cytochromesb ₆ per cytochromef. Cytochromef titrated as a single-electron acceptor with a pH-independent midpoint potential of +339 mV between pH 6.5 and 8.3, while cytochromeb ₆ was heterogeneous. With the assumption of two components present in equal amounts, two one-electron transitions withE _m(1)=–40 mV andE _m(2)=–172 at pH 6.5 were derived. Both midpoint potentials were pH-dependent.Abbreviation Tris tris(hydroxymethyl)aminomethane - SDS sodium dodecylsulfate - SDS-PAGE SDS polyacrylamide gel electrophoresis - MES 2-(N-morpholino)ethanesulfonic acid     

Organization and nucleotide sequence of the atp genes encoding the ATP synthase from alkaliphilic Bacillus firmus OF4

Summary The atp operon from the extreme alkaliphile Bacillus firmus OF4 was cloned and sequenced, and shown to contain genes for the eight structural subunits of the ATP synthase, preceded by a ninth gene predicted to encode a 14 kDa hydrophobic protein. The arrangement of genes is identical to that of the atp operons from Escherichia coli, Bacillus megaterium, and thermophilic Bacillus PS3. The deduced amino acid sequences of the subunits of the enzyme are also similar to their homologs in other ATP synthases, except for several unusual substitutions, particularly in the a and c subunits. These substitutions are in domains that have been implicated in the mechanism of proton translocation through F₀-ATPase, and therefore could contribute to the gating properties of the alkaliphile ATP synthase or its capacity for proton capture.     

The wild-type allele of tonB in Escherichia coli is dominant over the tonB1 allele, encoding TonBQ160K, which suppresses the btuB451 mutation

The entire coding sequence of the tonB gene, except for nine codons at the 3 end, was deleted from the chromosome of Escherichia coli. Introduction of the btuB451 suppressor mutant tonB1 into the chromosome of such a tonB deletion strain showed that the tonB1 allele was active as a suppressor in a single copy at 37° C and 42° C but not at 28° C. No temperature dependence was seen when FepA- or FhuA-dependent activities of the tonB1 gene product (TonB_Q160K) were tested. The btuB451 suppressor activity of tonB1 was inhibited by the simultaneous presence within the cells of the tonB ⁺ allele on a multicopy plasmid. This represents the first case of dominance among different tonB alleles. Inhibition of suppression was abolished by overexpression of the btuB451-encoded receptor protein. Competition for binding of TonB⁺ and TonB_Q150K to ExbB was excluded as the cause of dominance. Based on our data we conclude that competition for binding of TonB ⁺ and TonB_Q160K to the btuB451 gene product is the reason for the observed dominance. The implications of these findings for the mechanism of btuB451 suppression by tonB1 are discussed.