新疆雪莲体细胞胚胎发生

通过体细胞胚胎发生途径实现了新疆雪莲(Saussurea involucrata Kar.et Ki r.)的植株再生。选用新疆雪莲子叶为外植体, 接种于MS+0.5 mg.L-1 2,4-D+0.05-1 mg.L-1 BA的固体培养基上, 进行愈伤组织的诱导。从第1次继代培养的愈伤组织中挑选出黄绿色、颗粒状、质地致密的胚性愈伤组织, 转移到含0.05-0.1 mg.L-1 2,4-D 的MS液体培养基中进行悬浮培养,20天后可分化产生大量球形胚。继代过程中相继加入PEG和GA3 , 可以促进体细胞胚的分化和生长。体细胞胚在含有5 mg.L-1 GA3 的MS固体培养基上, 可发育成完整的植株。     

蓝花丹二型花雌、雄蕊发育进程及内源激素对花柱生长的影响

为了解二型花雌、雄蕊发育进程及内源激素对长、短花柱生长发育的影响,以蓝花丹(Plumbago auriculata Lam.)为材料,观察分析了长花柱(L型)、短花柱(S型)花朵内雌、雄蕊的发育特征,并分别检测了L、S型花柱中的内源激素水平。结果显示:蓝花丹雌、雄蕊发育进程基本符合逻辑斯蒂变化曲线,并可划分为5个时期,即T1初始发育期、T2转折期(一)、T3快速发育期、T4转折期(二)、T5平稳发育期;在整个发育进程中,L型花朵中雌蕊的生长速率始终高于雄蕊;S型花朵中雌蕊的生长速率在T3期由快转慢,导致T3~T5期雌蕊的生长速率始终低于雄蕊,从而形成了雌蕊低于雄蕊的短花柱特征。这说明花柱的分化是在二型花雌、雄蕊快速发育的T3期开始出现,并逐渐形成花柱异长植物最显著的花部形态特征。IAA、IPA和GA含量均在T1~T3期增加、T4~T5期降低,且在L型花柱中的含量始终高于S型,而ABA含量的变化趋势与这3种生长促进类激素相反,说明在蓝花丹花柱发育过程中,IAA、IPA和GA可能参与调控花柱的伸长生长,而ABA主要在发育后期促使花柱成熟。     

无籽西瓜发育过程中所需生长素来自何方?

答:高中生物(乙种本)第91页,讲到生长素促进果1993年第28卷第4期实发育时说:“胚珠发育成种子过程中,发育着的种子里合成大量的生长素。这些生长素能促进子房发育成果实。如果雌蕊受粉后,在子房发育成果实的早期,除去     

生长素信号转导途径与植物胁迫反应相互作用的证据

生长素影响植物多种生理过程,有报道显示生长素可能影响植物对逆境胁迫的反应.我们利用cDNA阵列技术鉴定拟南芥(Arabidopsis thaliana (L.) Heynh.)的生长素应答基因,发现多个胁迫应答基因受生长素抑制,包括Arabidopsis homolog of MEK kinase1 (ATMEKK1),RelA/SpoT homolog 3 (At-RSH3),Catalase 1 (Cat1) 和Ferritin 1 (Fer1),说明生长素可调节胁迫应答基因的表达.此外,我们还证明吲哚乙酸(IAA)合成途径中的腈水解酶基因nitrilase 1 (NIT1) 和nitrilase 2 (NIT2) 受盐胁迫诱导,提示在逆境条件下IAA的合成可能随之增加.我们利用生长素不敏感突变体研究生长素与逆境反应相互作用的信号转导,发现胁迫应答基因在野生型和生长素不敏感突变体auxin resistant 2 (axr2) 中可被盐胁迫诱导,而在auxin resistant 1-3 (axr1-3)中则不被诱导,说明生长素与逆境胁迫反应的相互作用可能发生在泛素途径.     

中华结缕草成熟胚的离体培养再生植株

1植物名称中华结缕草(Zoysia sinica). 2材料类别成熟种子. 3培养条件基本培养基为改良MS(MSm):MS无机盐 核黄素(VB2)1.0mg·L-1(单位下同) 盐酸噻胺(VB1)1.0 烟酸(Vpp)0.5 盐酸吡哆辛(VB6)0.5 肌醇100 酶水解酪蛋白(CH)300 蔗糖30 g.L-1 琼脂6.0 g·L-1.愈伤组织诱导培养基:(1)MSm4葡萄糖20 g·L-1 2,4-D 2.5 6-BA 0.25;愈伤组织继代培养基:(2)MSm 6-BA 0.1 2,4-D 1.6,(3)MSm 6-BA 0.1 2,4-D 2.0,(4)MSm 6-BA 0.1 2,4-D 2.4,(5)MSm 6-BA 0.1 2,4-D 2.8,(6)MSm 6-BA 0.1 2,4-D 3.2;分化培养基:(7)MSm.愈伤组织诱导和继代培养均为黑暗条件,分化培养过程中光照度为2000 lx,光照时间为12 h.d-1,培养温度(26±2)℃.     

大豆未成熟胚培养中高浓度植物生长素的作用及其植株再生

用大豆(Glycine max(L.)Merr.)未成熟胚为外植体,在含高浓度 NAA 或2,4-D 的培养基上可诱导绿色结构体和体细胞胚状体。叶状、花状和喇叭形状的绿色结构体在含30mg/l2,4-D 的 MS-1培养基上可重新愈伤组织化。这种由高浓度2,4-D 诱发并保持的愈伤组织,转到低激素水平的培养基上后,能诱导出大量的同类形状的新结构体。绿色结构体可以进一步发育成叶丛状,但顶端不伸长。使用含2m g/l GA,和0.1mg/l IBA 的培养基,能促进顶端伸长和根的发育,获得正常植株。由未成熟胚的子叶(其时种子长度约4—6mm)诱导的愈伤组织具有再生能力。在含高浓度2,4-D(5-30mg/l)的培养基上诱导出的愈伤组织具有较高的产生绿色结构的潜力。而高浓度 NAA(10mg/l)培养基产生的愈伤组织具有较强的产生根状体的潜力。培养的外植体或愈伤组织在含5mg/l 2,4-D 的培养基上,不需要经常的继代培养,即可长期保存。     

生长素和乙烯互作调控硝酸铵诱导的根毛分叉

以野生型拟南芥(WT)及其生长素和乙烯不敏感型突变体(aux1-7、axr1-3、etr1-1和etr1-3)为实验材料,采用固体培养法研究了高浓度硝酸铵对根毛发育的影响,以揭示其调控根毛发育的机制。结果表明:(1)随着外源硝酸铵浓度的逐渐增加,拟南芥根毛伸长受阻,产生大量的分叉根毛。(2)高浓度硝酸铵条件下,外源活性氧或活性氧产生抑制剂二苯基氯化碘(DPI)的添加能抑制高浓度硝酸铵诱导的分叉根毛产生。(3)高浓度硝酸铵条件下,外源生长素或乙烯合成前体物质1-氨基-环丙烷-1-羧酸(ACC)处理能恢复根毛的正常生长,解除高浓度硝酸铵诱导根毛分叉现象。(4)高浓度硝酸铵条件下,外源生长素处理乙烯不敏感型突变体或ACC处理生长素不敏感型突变体均能抑制突变体分叉根毛的形成。研究表明,活性氧、生长素和乙烯都参与了高浓度硝酸铵对根毛发育的过程调控;在硝酸铵诱导的根毛分叉中生长素和乙烯存在相互作用,在缺乏生长素信号通路时,乙烯能够发挥补充作用抑制分叉根毛的产生;在缺乏乙烯信号通路时,生长素也可以弥补缺失乙烯的作用抑制根毛的分叉,但是需要更高浓度的生长素才能充分抑制分叉根毛的产生。     

石刁柏花药培养诱导成完整植株

植物名称:石刁柏(Asparagus officinalis),品种为玛丽华盛顿500(Mary Washington 500)。材料类别:长度为1.5～2.0mm(从花萼基部到顶端)的花蕾,接种花粉发育时期为单核的中、晚期花药(醋酸洋红压片法镜检),色呈浅黄。培养条件:诱导愈伤组织培养基:MS附加(1)NAA0.2mg/l(单位下同) BA0.5 2,4-D1.0;(2)NAA0.4 BA0.2 2,4-D1.0;(3)NAA0.1 BA0.2 2,4-D1.5;(4)NAA0.1 BA0.2 2,4     

Proliferation and differentiation from endosperms of Carthamus tinctorius

The endosperms of Carthamus tinctorius cv. HUS-305, excised at globular to heart-shaped stages of zygotic embryo development, were cultured on Murashige and Skoog’s medium (MS) supplemented with different concentrations of 6-benzylaminopurine (BAP), kinetin, thidiazuron (TDZ), 2,4-dichlorophenoxyacetic acid (2,4-D) or α-naphthalene-acetic acid (NAA). The highest incidence of callusing was on 2,4-D supplemented media. However, embryos differentiated only from the calli developed on media supplemented with BAP, kinetin or TDZ with the last eliciting maximum embryogenic response. The addition of a reduced nitrogen source, casein hydrolysate to MS medium supplemented with BAP and/or NAA, did not stimulate the response. However, adenine sulphate (100 mg dm⁻³) promoted the induction of somatic embryos. Upon transfer to MS basal medium or the same supplemented with 0.61 μM gibberellic acid (GA₃), plumular poles of few embryos elongated resulting in the development of shoots.     

东南景天的组织培养和快速繁殖

1 植物名称 东南景天（Sedum alfredii Hance）. 　　2 材料类别 幼嫩叶片. 　　3 培养条件 基本培养基为MS.（1）愈伤组织诱导培养基：MS＋6-BA 0.1 mg·L-1（单位下同）＋2,4-D1.0～3.0;（2）愈伤组织继代培养基：MS＋6-BA 0.1＋2,4-D 1.0＋VC 2.0＋1.0 g·L^-1活性炭;（3）分化培养基：MS＋6-BA 2.0＋2,4-D 1.0＋AgNO4 2.0;（4）壮苗培养基：MS＋6-BA 0.1＋GA3 2.0;（5）生根培养基：1/3MS＋NAA 1.0.以上培养基中均加入12g·L^-1琼脂、30 g·L^-1蔗糖,pH 5.6～5.8,在智能型光照培养箱（MGC-300B型,上海一恒科技有限公司）内培养.光照时间16 h·d^-1,光照强度为40～60 μmol·m^-2·s^-1,培养温度为（25±1）℃.[第一段]     

Differential Hypocotyl and Root Development of Arabidopsis Auxin-Insensitive Mutants

Arabidopsis , aux1-7, axr1-3 and axr2-1, grown in a natural sandy soil, without sucrose supplementation. The three mutants showed impaired epidermal cell elongation in the hypocotyls of 15-day-old seedlings, with axr2-1 showing the most marked effects. In addition, the roots of axr2-1 elongated faster and presented a more extended meristematic zone than the other genotypes. Unchanged epidermal cell length in the differentiation zone of axr2-1 relative to the wild-type suggested enhancement of cell proliferation. These alterations may have affected the timing and site of emergence of the root hairs, starting later and further from the root tip than in the other genotypes. Similarly to the wild-type, no root hair growth was initiated in axr2-1 drought-induced short roots, although the epidermis was differentiated into trichoblasts and atrichoblasts. On rehydration of the short roots, hair formation occurred from trichoblasts prior to epidermal cell elongation. Therefore, auxin-insensitivity in the axr2-1 mutant did not result in alterations of the hair-forming process itself. The differential development of axr2-1 seedlings, relative to the other auxin-insensitive mutants, suggested that the AXR2 gene has a complex, regulatory function in multiple hormone signaling. Received 26 July 2000/ Accepted in revised form 28 February 2001     

Novel software for analysis of root gravitropism: comparative response patterns of Arabidopsis wild-type and axr1 seedlings

In an earlier study (Evans, Ishikawa & Estelle 1994, Planta 194, 215-222) we used a video digitizer system to compare the kinetics of auxin action on root elongation in wild-type seedlings and seedlings of auxin response mutants of Arabidopsis thaliana (L.) Heynh. We have since modified the system software to allow determination of elongation on opposite sides of vertical or gravistimulated roots and to allow continuous measurement of the angle of orientation of sequential subsections of the root during the response. We used this technology to compare the patterns of differential growth that generate curvature in roots of the Columbia ecotype and in the mutants axr1-3, axr1-12 and axr2, which show reduced gravitropic responsiveness and reduced sensitivity to inhibition by auxin. The pattern of differential growth during gravitropism differed in roots of wild-type and axr1 seedlings. In wild-type roots, initial curvature resulted from differential inhibition of elongation in the distal elongation zone (DEZ). This was followed by an acceleration of elongation along the top side of the DEZ. In roots of axr1-3, curvature resulted from differential stimulation of elongation whereas in roots of axr1-12 the response was variable. Roots of axr2 did not exhibit gravitropic curvature. The observation that the pattern of differential growth causing curvature is dramatically altered by a change in sensitivity to auxin is consistent with the classical Cholodny-Went theory of gravitropism which maintains that differential growth patterns induced by gravistimulation are mediated primarily by gravi-induced shifts in auxin distribution. The new technology introduced with this report allows automated determination of stimulus response patterns in the small but experimentally popular roots of Arabidopsis.     

Interaction of jasmonic acid and blue light in the regulation of arabidopsis morphogenesis

The effects of blue light (BL) and jasmonic acid (JA) on morphogenesis of Arabidopsis thaliana (L.) Heynh seedlings of genotypes Col and Ler and their mutants, namely, axr1-3 and jar1-1 mutants resistant to IAA and JA, respectively, and a CRY1 photoreceptor-deficient mutant hy4 were studied. Both 1 μM JA and BL exposure retarded hypocotyl growth of Ler, Col, and jar1-1 seedlings, whereas JA had no effect on hypocotyl growth of axr1-3, but the suppression of hypocotyl growth of this mutant by BL was even more noticeable than that of Ler, Col, and jar1-1. JA and BL applied simultaneously inhibited hypocotyl growth of axr1-3 and especially of Ler, Col, and jar1-1 more than either of factors applied separately. The hy4 mutant did not respond to BL, whereas JA stimulated its hypocotyl growth. JA did not change the cotyledon size of Col, axr1-3, and jar1-1 and reduced the cotyledon size of Ler and hy4. BL enhanced the cotyledon growth of all wild-type and mutant plants used in the study. The cotyledon sizes of all plants except Ler were also increased when JA and BL were applied together. Some of the growth responses correlated with the endogenous IAA and ABA contents. Thus, for example, the hypocotyl and cotyledon growth retardation of Ler seedlings in the presence of JA correlated with a reduced level of free IAA and a considerable increase in the free ABA level in plants grown both in darkness and in BL. Under other growth conditions, no correlation between the endogenous IAA and ABA levels and A. thaliana seedling growth was noted. The interaction between the signal transduction pathways triggered by BL and JA at the early stages of arabidopsis morphogenesis is discussed on the basis of Col, Ler, axr1-3, and jar1-1 hypocotyl growth responses.     

一种新融合抗菌肽Hex-Mag基因的克隆、表达及其抗菌活性的研究

通过在Magainin1-12(GIGKFLHSAKKF)的N端添加碱性氨基酸片段Hexapeptide(RRWQWR)以增强其对细胞膜的吸附能力来提高Magainin1-12的抗菌活性。利用Hexapeptide和Magainin1-12的基因序列,结合酵母偏爱密码子设计出新的融合基因Hex-Mag,通过重叠区扩增基因拼接法(Gene splicing by overlap extension,gene SOEing)利用PCR扩增出基因片段,再将融合基因进行酶切并纯化后导入穿梭质粒pPIC9中,构建受乙醇氧化酶1基因(AOX1)的启动子与转录终止区控制的酵母表达质粒,转化GS115毕赤酵母宿主菌,经表型筛选,阳性克隆用甲醇诱导表达。表达出的融合肽Hex-Mag分子量约2.3kDa,其耐热性强,在100℃条件下,其活性可维持3h以上。琼脂糖孔穴扩散法检测显示Hex-Mag对多种革兰氏阴性菌和阳性菌具有抑制活性,与Magainin1-12相比,其活性有明显增强,N端正电荷增加的预期效应得到初步体现。     

Neurite formation and membrane changes of mouse neuroblastoma cells induced by valinomycin

A clonal cell line of mouse neuroblastoma cells was found to undergo morphological differentiation in the presence of a K⁺ ionophore, valinomycin, in the assay medium. This effect was blocked by increasing the concentration of KCl of the medium, suggesting that the changes in resting membrane potential and ion fluxes may be involved in the mechanism of the formation of neurites. No enhancement of the neurite formation was observed in salines containing high concentrations of KCl in the absence of valinomycin. Depolarizing agents including veratridine, gramicidin and ouabain did not stimulate the outgrowth of neurites. Neither electrophoretic mobility of the cells nor molecular anisotropy of fluorescence probes in the membranes was modified by the treatment of valinomycin. Instead, it modified the slow binding phase in kinetics of the interaction of 1-anilinonaphthalene-8-sulfonate (ANS) with the cells, which is related to the penetration process of the probe into membranes. Valinomycin also enhanced the fluorescence intensity of ANS by increasing the binding sites in neuroblastoma cells.     

新型的干扰素λ家族

干扰素λ为一类新型的干扰素家族,分IFN-λ1、IFN-λ2和IFN一λ3等3种,也分别称为IL-29,IL-28A和IL-28B;其功能受体复合物是由新鉴定的CRF2—12和IL-10R2组成的异二聚体。配体与受体相互作用能活化Jak—STAT通路,并起抗病毒或其他防御功能作用。     

Mapping the interaction of bradykinin 1-5 with the exodomain of human protease activated receptor 4

The angiotensin converting enzyme breakdown product of bradykinin, bradykinin 1-5 (RPPGF), inhibits thrombin-induced human or mouse platelet aggregation. RPPGF binds to the exodomain of human protease-activated receptor 1 (PAR1). Studies determined if RPPGF also binds to the exodomain of human PAR4. RPPGF binds to a peptide of the thrombin cleavage site on PAR4. Recombinant wild-type and mutated exodomain of human PAR4 was prepared. The N-terminal arginine on RPPGF binds to the P2 position or proline46 on PAR4 to block thrombin cleavage. These data indicate that RPPGF influences thrombin activity by binding to the thrombin cleavage site on both PAR4 and PAR1.     

The presence of a Sar1 gene family in Brassica campestris that suppresses a yeast vesicular transport mutation Sec12-1

Two new members (Bsar1a and Bsar1b) of the Sar1 gene family have been identified from a flower bud cDNA library of Brassica campestris and their functional characteristics were analyzed. The two clones differ from each other at 14 positions of the 193 amino acid residues deduced from their coding region. The amino acid sequences of Bsar1a and Bsar1b are most closely related to the Sar1 family, genes that function early in the process of vesicle budding from the endoplasmic reticulum (ER). The sequences contain all the conserved motifs of the Ras superfamily (G1–G4 motifs) as well as the distinctive structural feature near the C-terminus that is Sar1 specific. Our phylogenetic analysis confirmed that these two clones can indeed be considered members of the Sar1 family and that they have a close relationship to the ARF family. The Bsar1 proteins, expressed in Escherichia coli, cross-reacted with a polyclonal antibody prepared against Saccharomyces cerevisiae Sar1 protein. It also exhibited GTP-binding activity. Genomic Southern blot analysis, using the 3'-gene-specific regions of the Bsar1 cDNAs as probes, revealed that the two cDNA clones are members of a B. campestris Sar1 family that consists of 2 to 3 genes. RNA blot analysis, using the same gene-specific probes, showed that both genes are expressed with similar patterns in most tissues of the plant, including leaf, stem, root, and flower buds. Furthermore, when we placed the two Bsar1 genes under the control of the yeast pGK1 promoter into the temperature-sensitive mutant yeast strain S. cerevisiae Sec12-1, they suppressed the mutation which consists of a defect in vesicle transport. The amino acid sequence similarity, the GTP-binding activity, and the functional suppression of the yeast mutation suggest that the Bsar1 proteins are functional homologues of the Sar1 protein in S. cerevisiae and that they may perform similar biological functions.