蓝莓玻璃化试管苗的显微结构及生理生化特性变化

研究了蓝莓试管苗玻璃化的显微结构、超微结构以及生理生化特性的影响。与正常试管苗相比,蓝莓玻璃化苗的茎、叶显微结构发生了明显的改变：叶片表皮细胞松散、不连续;气孔结构难以辨认;叶片增厚;缺少栅栏组织,海绵组织细胞间隙变大,部分细胞解体;茎的维管组织发育不良;亚显微结构观察发现,玻璃化苗叶肉细胞体积增大,细胞壁变薄;部分细胞缺少细胞核及线粒体;叶绿体数目减少,类囊体解体,缺乏淀粉体。玻璃化试管苗的生理生化特性也发生了显著的改变：玻璃化苗组织含水量显著增加;叶绿素、可溶性糖及可溶性蛋白含量显著降低;O2- 产生速率、H2O2积累量、MDA含量及相对电导率显著升高;活性氧清除酶系中POD活性显著升高,SOD和CAT活性显著降低;PAL活性下降。蓝莓玻璃化苗的形态结构异常,水分及物质代谢紊乱,活性氧清除能力降低,表明玻璃化与氧化胁迫相关。     

H2O2胁迫锻炼对小麦幼苗抗旱性的影响

12 d龄的春小麦幼苗在1 mmol·L-1 及10 mmol·L-1 H2O2的胁迫锻炼过程中,质膜透性增大,O-·及H2O2含量增多,CAT活性升高,叶绿素含量降低,低浓度H2O2胁迫使SOD活性上升,高浓度时却使其活性下降.经过H2O2胁迫锻炼后的小麦遭受干旱胁迫时,叶绿素含量、SOD活性、CAT活性均高于对照组,而质膜透性、O-·及H2O2含量却低于对照组.表明H2O2胁迫锻炼,提高了小麦幼苗的抗氧化能力,增强了其抗旱性.     

外源亚精胺对Hg2+胁迫下凤眼莲抗氧化系统的影响

通过Hoagland溶液培养实验,研究了外源亚精胺(Spd)(0.1 mmol?L-1)对Hg2+(0、10、20、30和40μmol?L-1)胁迫下凤眼莲叶片细胞内叶绿素、可溶性糖、可溶性蛋白含量及抗氧化系统的调节作用.结果显示,(1)随Hg2+处理浓度的升高,各处理凤眼莲叶片叶绿素a(Chl a)和叶绿素b(Chl b)含量均先升后降,并均在10μmol?L-1时达到最高值,但外源Spd处理组显著高于相应对照.(2)各处理凤眼莲叶片可溶性蛋白含量随Hg2+处理浓度的升高也呈先升后降趋势,而可溶性糖含量则呈持续上升趋势,但外源Spd处理亦明显高于相应对照.(3)随Hg2+处理浓度的升高,抗氧化物质AsA和GSH含量及抗氧化酶SOD、CAT、POD、APX及GR活性也均呈先升后降的变化趋势,而外源Spd处理植株的含量和活性均显著高于相应对照.(4)各处理凤眼莲叶片的H2O2、MDA含量及O2?-产生速率随Hg2+处理浓度的升高均持续上升,但在外源Spd处理后均比对照组下降.研究表明,Hg2+胁迫使凤眼莲生长受到严重伤害,外源Spd可大幅度地提高其抗氧化物质含量和保护酶活性,从而增强凤眼莲抗Hg2+胁迫的能力.     

镉胁迫下绿豆和箭舌豌豆幼苗的抗氧化反应

采用溶液培养法对Cd2 胁迫下绿豆和箭舌豌豆幼苗叶组织内的抗氧化酶活性、活性氧和丙二醛(MDA)含量以及细胞电解质泄漏率的变化进行了研究。结果显示,随着Cd2 胁迫浓度的增加和胁迫时间的延长,2种作物叶组织内的MDA含量和细胞电解质泄漏率明显增加;在胁迫期间,二者的过氧化氢(H2O2)和超氧阴离子(O2.-)的含量以及过氧化氢酶(CAT)、抗坏血酸过氧化物酶(APX)、超氧化物歧化酶(SOD)活性呈先升高并在不同的时间达到高峰后再下降的趋势。与箭舌豌豆相比,Cd2 胁迫下的绿豆幼苗叶组织的MDA含量、电解质泄漏率及H2O2和O2.-的积累量较高,CAT、SOD和APX的活性较低。研究表明,Cd2 胁迫下箭舌豌豆的抗氧化能力高于绿豆的抗氧化能力。     

外源GSH对盐胁迫下番茄幼苗生长及抗逆生理指标的影响

采用营养液栽培法,研究外源谷胱甘肽(GSH)对NaCl胁迫下番茄幼苗生长、根系活力、电解质渗透率和丙二醛(MDA)、脯氨酸(Pro)、可溶性糖含量以及超氧化物歧化酶(SOD)、过氧化物酶(POD)、过氧化氢酶(CAT)活性的影响,为利用外源物质减轻盐胁迫伤害提供理论依据。结果显示:(1)NaCl胁迫显著抑制了番茄幼苗的生长、根系活力和SOD、POD、CAT活性,提高了电解质渗透率及MDA、Pro、可溶性糖含量;(2)外源喷施GSH能够诱导NaCl胁迫下番茄幼苗叶片抗氧化酶SOD、POD、CAT活性上调,电解质渗透率及MDA含量下降,Pro和可溶性糖含量恢复至对照水平;(3)外源喷施还原型谷胱甘肽抑制剂(BSO)使NaCl胁迫下番茄幼苗的根系活力以及抗氧化酶SOD、POD、CAT活性下降,脯氨酸含量提高;(4)喷施GSH可诱导BSO和NaCl共处理番茄植株的根系活力、SOD、POD、CAT活性提高,MDA和Pro含量降低。研究表明,外源GSH可通过提高促进盐胁迫下番茄幼苗植株渗透调节能力及清除活性氧的酶促系统的防御能力、降低细胞膜脂过氧化程度、保护膜结构的完整性,从而有效缓解NaCl胁迫对番茄幼苗生长的抑制,提高其耐盐性。     

外源ABA对大蒜试管苗玻璃化发生和抗氧化系统的影响

以大蒜品种‘二水早’试管苗为材料,从活性氧代谢的角度研究了外源ABA、H_2O_2和H_2O_2+ABA处理下的试管苗玻璃化率、活性氧积累与组织定位和抗氧化系统的响应特征,探讨ABA缓解试管苗玻璃化过程的机理。结果表明:(1)外源H_2O_2处理可诱导大蒜试管苗玻璃化发生,外源ABA处理下玻璃化率最低,可以缓解H_2O_2诱导的玻璃化的发生。(2)试管苗O_2~产生速率和H_2O_2含量在H_2O_2处理下最高,在ABA处理下最低;在添加H_2O_2的培养基中同时添加ABA能显著减少因外源H_2O_2处理引起的O_2~产生和H_2O_2积累。(3)试管苗CAT、POD和APX活性在外源H_2O_2处理前期(0~8d)均上升并显著高于对照,但其CAT、APX活性在处理后期(8~16d)下降,其同期POD活性也增加缓慢;各抗氧化酶的活性在外源ABA与H_2O_2+ABA处理前期(0~8d)均呈直线上升趋势,而它们在H_2O_2+ABA处理后期(8~16d)均显著高于H_2O_2处理。(4)各处理试管苗抗坏血酸和谷胱甘肽含量随处理时间先升高后降低,并以外源ABA处理下最高,外源H_2O_2处理下最低。(5)试管苗O_2~和H_2O_2产生部位主要在基部和叶尖,且外源ABA处理下组织中ROS的积累最少。(6)在ABA+H_2O_2处理下,大蒜试管苗内丙二醛含量和膜相对透性显著低于对照和H_2O_2处理。研究发现,外源ABA处理可有效降低大蒜试管苗的内源O_2~产生速率和H_2O_2含量,提高抗氧化酶活性和抗氧化物质含量,抑制活性氧在试管苗内的产生和运输,显著降低试管苗玻璃化率;外源ABA可通过增强大蒜试管苗抗氧化能力来抑制玻璃化发生。     

H_2O_2胁迫锻炼对小麦幼苗抗旱性的影响

12 d龄的春小麦幼苗在 1 mmol· L- 1及 1 0 mmol· L- 1H2 O2 的胁迫锻炼过程中 ,质膜透性增大 ,O- · 及 H2 O2 含量增多 ,CAT活性升高 ,叶绿素含量降低 ,低浓度 H2 O2 胁迫使SOD活性上升 ,高浓度时却使其活性下降。经过 H2 O2 胁迫锻炼后的小麦遭受干旱胁迫时 ,叶绿素含量、SOD活性、CAT活性均高于对照组 ,而质膜透性、O- · 及 H2 O2 含量却低于对照组。表明 H2 O2 胁迫锻炼 ,提高了小麦幼苗的抗氧化能力 ,增强了其抗旱性     

美丽箬竹对模拟大气O3浓度倍增胁迫的生理响应

运用开顶式气室(OTCs)模拟当前环境大气O3浓度(对照,40～45 nL·L-1)、O3浓度倍增4倍(TR-1,92～106 nL·L-1)和O3浓度倍增2倍(TR-2,142～160 nL·L-1)胁迫,以叶片光合色素、MDA、可溶性蛋白质和可溶性糖含量及SOD和POD活性和相对电导率为指标,分析了美丽箬竹(Indocalamus decorus Q.H.Dai)对O3胁迫的生理响应规律.结果显示:随O3浓度的提高,叶片叶绿素a(Chla)、叶绿素b(Chlb)、总叶绿素和类胡萝卜素含量,SOD和POD活性,可溶性蛋白质和可溶性糖含量及二者的比值(SPC/SSC)均呈下降趋势;叶绿素a口与b的比值(Chla/Chlb)、MDA含量和相对电导率均呈增加趋势.TR-1条件下叶片POD活性和可溶性糖含量分别比对照下降38.86％和10.37％,差异显著;Chla/Chlb比值显著高于对照,其余指标均与对照无显著差异.而在TR-2条件下叶片Chla、Chlb、总叶绿素和类胡萝卜素含量显著低于对照,降幅分别为26.89％、40.91％、30.47％和20.37％;SOD和POD活性、可溶性蛋白质和可溶性糖含量以及PC/SSC比值也均显著低于对照,降幅分别为42.03％、46.62％、45.09％、11.52％和40.15％;Chla/Chlb比值、MDA含量和相对电导率均显著高于对照.另外,TR-1与TR-2处理组间光合色素含量和POD活性差异不显著,TR-2处理组MDA含量和相对电导率显著高于TR-1处理组,SOD活性显著低于后者.研究结果表明:美丽箬竹对O3胁迫具有强耐受性,可种植于O3浓度较高的环境中.     

大蒜叶片活性氧及保护酶系对白腐病菌粗毒素胁迫的响应

以大蒜抗病品种‘汉中红皮’和感病品种‘改良蒜’为材料,研究了它们在苗期用白腐病菌毒素处理后的叶片细胞超氧化物歧化酶(SOD)、过氧化物酶(POD)和过氧化氢酶(CAT)活性以及超氧阴离子(O2-.)和丙二醛(MDA)含量的动态变化。结果表明,白腐病菌粗毒素处理后,2个品种大蒜叶片的SOD、POD活性均升高,而CAT活性降低;抗病品种的SOD、POD和CAT活性均高于感病品种,且SOD、POD活性峰值出现早,并以POD对毒素胁迫最敏感。2个品种在白腐病菌粗毒素处理后的O2.-含量始终高于同期对照,而感病品种O2.-含量在毒素处理24h后均高于同期抗病品种。MDA含量变化趋势与O2.-的变化基本相似。研究认为,大蒜叶片的活性氧含量和保护酶活性与其抗病性密切相关。     

香蒲对不同浓度Pb~(2+)胁迫的生理应答及其细胞超微结构变化

通过室内水培试验,研究了不同浓度Pb2+(0、0.25、0.50、1.00和2.00mmol·L-1)胁迫对东方香蒲根和叶中Pb含量、叶绿素含量、丙二醛(MDA)含量、抗氧化酶(SOD、CAT和POD)活性以及亚细胞结构的影响。结果显示:(1)随着外源Pb2+浓度的增加,Pb在香蒲根和叶中的积累量均显著高于对照,且Pb在根中的含量明显高于叶中,并与外源Pb2+浓度呈显著正相关关系。(2)香蒲叶片中的叶绿素a和叶绿素b含量随着外源Pb2+浓度的增加呈先升后降趋势,均在处理浓度为0.50mmol·L-1时达到峰值。(3)胁迫处理叶片的MDA含量与对照相比变化不显著,但根中MDA含量呈显著下降趋势。(4)叶片中SOD活性在1.00mmol·L-1 Pb2+处理时达到峰值,然后下降,但始终高于对照,CAT和POD活性则均低于对照组;根中SOD活性除1.00mmol·L-1 Pb2+处理组外均显著低于对照组,CAT和POD活性分别在0.25和0.50mmol·L-1 Pb2+处理时达到峰值,然后随处理Pb2+浓度升高而下降。(5)电镜观察发现,Pb2+胁迫使香蒲叶细胞中叶绿体被膜破裂,类囊体膨胀、破损;根和叶细胞中的线粒体被膜均破裂、内腔空泡化,细胞核核膜破损、核仁消失、染色质凝集。研究表明,Pb2+胁迫致使东方香蒲根、叶生理代谢失衡,亚细胞结构出现不可逆的损伤,这为从分子水平研究Pb2+作用的具体机理以及香蒲在重金属污染修复中的应用提供了依据。     

Synthesis and physicochemical properties of 2'-deoxy-2',2'-difluoro-beta-D-ribofuranosyl and 2'-deoxy-2',2'-difluoro-alpha-D-ribofuranosyl oligonucleotides

We present procedures for nucleoside and oligonucleotide synthesis, binding affinity (Tm) and structural analysis (CD spectra) of 2'-deoxy-2',2'-difluoro-alpha-D-ribofuranosyl and 2'-deoxy-2',2'-difluoro-beta-D-ribofuranosyl oligothymidylates. Possible reasons for the thermal instability of duplexes formed between these compounds and RNA or DNA targets are discussed.     

BCL2-CISD2

CISD2, an ER BCL2-associated autophagy regulator also known as NAF-1, is responsible for the human degenerative disorder Wolfram Syndrome 2. In order to interrogate the physiological role of CISD2 we generated and characterized the Cisd2 gene deletion in mice. Cisd2 null mice manifest significant degeneration in skeletal muscle tissues, which is accompanied with augmented autophagy, dysregulated Ca²⁺ homeostasis and elongated mitochondria. Our findings describe a novel role for BCL2-CISD2 in the homeostatic maintenance of skeletal muscle. It remains to be elucidated how and if the antagonism of the BECN1 autophagy-initiating complex and modulation of ER Ca²⁺ homeostasis by BCL2-CISD2 are interconnected.     

Synthesis of [11-2H2], [8-2H2], [7-2H2], [6-2H2], [5-2H2], [4-2H2] and [3-2H2] cis-9-octadecenoates

Deuterated oleates have been synthesized by semihydrogenation of acetylenic intermediates. [11-²H₂]Oleate was prepared by two-carbon chain extension of the C₁₆ alcohol obtained from [1-²H₂]octyl bromide and 7-octyn-1-ol. [8-²H₂] and [7-²H₂]oleates were both prepared from dimethyl suberate, tetradeutero intermediate C₁₆ alcohols were synthesized from [1,8-²H₄] and [2,7-²H₄]octane diols by monobromination, conversion to deuterated 9-decyn-1-ols and reaction with octyl bromide. Oxidation gave [8-²H₂]-9-octadecynoate and [2,7-²H₂]-9-octadecynoate, after semihydrogenation of the latter, deuterons at C-2 were removed by exchange with aqueous alkali. [6-²H₂] and [5-²H₂]oleates were obtained from methyl 5-tetradecynoate, semihydrogenation, deuterium exchange at C-2 and two malonate extensions gave [6-²H₂]oleate; reduction with lithium aluminum deuteride, two malonate extensions and semihydrogenation gave the [5-²H₂] ester. [4-²H₂] and [3-²H₂]oleates were both obtained from methyl 7-cis-hexadecenoate, exchange of the α protons and chain extension gave the [4-²H₂] ester and reduction with lithium aluminum deuteride and chain extension gave the [3-²H₂] ester.     

Stereospecific 2'-amination and 2'-chlorination of adenosine by Actinomadura in the biosynthesis of 2'-amino-2'-deoxyadenosine and 2'-chloro-2'-deoxycoformycin

2'-Amino-2'-deoxyadenosine and 2'-chloro-2'-deoxycoformycin (2'-CldCF) are two nucleoside antibiotics produced by Actinomadura. The biosynthesis of these two nucleoside antibiotics has been studied by the addition of [U-14C]adenosine with or without unlabeled adenine to cultures of Actinomadura. By this experimental approach, it is possible to demonstrate that adenosine is the direct precursor for the biosynthesis of 2'-amino-2'-deoxyadenosine and 2'-CldCF. These conclusions are based on the observation that the percentage distribution of 14C in the aglyconic and pentofuranosyl moieties of 2'-amino-2'-deoxyadenosine and 2'-CldCF were similar to the distribution of 14C in the adenine and ribosyl moieties of the [U-14C]adenosine (i.e., 48:52) added to cultures of Actinomadura. Experimentally, the percentage distribution of 14C in the (i) adenine:2-amino-2-deoxy-beta-D-ribofuranose of 2'-amino-2'-deoxyadenosine is 51:49; (ii) 8-(R)-3,6,7,8-tetrahydroimidazo[4,5-d]-[1,3-diazepin-8-o1]:2 -chloro-2- beta-D-ribofuranose of 2'-CldCF is 45:55; and (iii) adenine:ribose of the adenosine isolated from the RNA of Actinomadura is 42:58. Further proof that adenosine is the direct precursor for the biosynthesis 2'-amino-2'-deoxyadenosine and 2'-CldCF was demonstrated by the addition of 75 mumol of unlabeled adenine together with [U-14C]adenosine to nucleoside-producing cultures of Actinomadura. The percentage distribution of 14C in the aglycon and the sugar moieties of 2'-amino-2'-deoxyadenosine and 2'-CldCF were 46:54 and 47:53, respectively; the percentage distribution of 14C in the adenine and ribose moieties of the adenosine isolated from the RNA of Actinomadura was 51:49. These data show that the hydroxyl on C-2' of the ribosyl moiety of adenosine undergoes a replacement by a 2'-amino or a 2'-chloro group to form 2'-amino-2'-deoxyadenosine or 2'-CldCF with retention of stereconfiguration at C-2'. Finally, Actinomadura can utilize inorganic chloride from the medium as demonstrated by the isolation of [36Cl]2'-CldCF following the addition of [36Cl]chloride to the culture medium. Mechanisms for the regioselective modification of the C-2' hydroxyl group and stereospecific insertion of the amino and chloro groups are discussed.     

Stereospecific formation of alpha-hydroxycarboxylato oxo peroxo complexes of vanadium(V). Crystal structure of (NBu4)2[V2O2(O2)2(L-lact)2] x 2H2O and (NBu4)2[V2O2(O2)2(D-lact)(L-lact)] x 2H2O

An overview of structurally characterized alpha-hydroxycarboxylatodioxo- and alpha-hydroxycarboxylatooxoperoxovanadates(V) is presented and the geometric parameters of the V2O2 bridging core are discussed. The first case of a stereospecific formation of oxoperoxovanadates(V) is reported: The crystal structures of the isomeric compounds (NBu4)2[V2O2(O2)2(L-lact)2] x 2H2O and (NBu4)2[V2O2(O2)2(D-lact)(L-lact)] x 2H2O (lact = C3H4O3(2-), the anion of the lactic acid) differ mainly in the arrangement of the V2O2 core and in mutual orientation of the V=O bonds. The complexes with achiral ligands adopt the same structural type as the complexes formed from a racemic mixture of a chiral ligand, while the structure obtained using an enantiopure L,L-hydroxycarboxylate is different.     

Convenient synthesis of 2'-deoxy-2-fluoroadenosine from 2-fluoroadenine

A convenient synthesis of 2'-deoxy-2-fluoroadenosine from commercially available 2-fluoroadenine is described. The coupling reaction of silylated 2-fluoroadenine with phenyl 3,5-bis[O-(t-butyldimethylsilyl)]-2-deoxy-1-thio-D-erythro-pentofuranoside gave the corresponding 2-fluoro-2'-deoxyadenosine derivative (alpha/beta = 1:1) in good yield. The alpha- and beta-anomers were separated by chromatography, and then desilylated to give compounds 1a and 1b.     

Synthesis and properties of 2'-O-methyl-2-thiouridine and oligoribonucleotides containing 2'-O-methyl-2-thiouridine

A new method for the synthesis of 2'-O-methyl-2-thiouridine (s2Um) found in thermophilic bacterial tRNA was developed. Structural properties of s2Um and s2Um(p)U were studied by using 1H NMR spectroscopy. A modified nonaribonucleotide (RNA*: 5'-CGUUs2UmUUGC-3') was synthesized to study the base-recognition ability of s2Um in formation of RNA-RNA and RNA DNA duplexes. The UV melting experiments revealed that RNA*-RNA and RNA*-DNA duplexes having an s2U-A base pair are more stable than those having a U-A base pair. On the contrary, the thermal stability of RNA*-RNA and RNA*-DNA duplexes having an s2U-G wobble base pair was much lower than that of the unmodified duplexes having a natural U-G base pair. It is concluded that s2Um has higher selectivity toward A over G than unmodified U.