果树花芽孕育的研究概况

果树花芽孕育是一个成花因素积累的过程,也是芽顶端花原基形成前所必要的活动。随着研究手段的改进和水平的提高,近年来人们逐渐弄清了果树花芽孕育的概念、花芽孕育期间的重要生理生化变化以及外界因素调控花芽孕育的可能方式,而对果树花芽孕育调控基因的研究处于起步阶段。     

激素信号在调节果树花芽发端假说的概述

概述了Lavee和Bangerth两个激素信号调节花芽发端假说的内容和证据,并分析了这两个假说的优缺点。认为旺盛营养生长的梢尖或正在发育果实的种子产生的极性运输的生长素（IAA）可能是抑制果树花芽发端的信号。尚不能确定来自正在发育果实种子的赤霉素（GA）自身是抑制花芽发端的信号,还是参与调节花芽发端信号的产生。营养芽中高水平的细胞分裂素（CTK）促进花芽发端,可能与较弱的IAA信号有关。同时指出,激素信号调节花芽发端的机理还有待完善。     

激素信号调节果树花芽发端假说的概述

概述了Lavee和Bangerth两个激素信号调节花芽发端假说的内容和证据,并分析了这两个假说的优缺点。认为旺盛营养生长的梢尖或正在发育果实的种子产生的极性运输的生长素（IAA）可能是抑制果树花芽发端的信号。尚不能确定来自正在发育果实种子的赤霉素（GA）自身是抑制花芽发端的信号,还是参与调节花芽发端信号的产生。营养芽中高水平的细胞分裂素（CTK）促进花芽发端,可能与较弱的IAA信号有关。同时指出,激素信号调节花芽发端的机理还有待完善。     

喷施烯效唑对苹果顶芽激素水平和花芽分化的影响

用烯效唑(uniconazol,S3307)1 g/L喷洒“红富士“苹果树降低了顶芽IAA、GA1,3,4,7含量,提高了ZR、ABA含量,从而提高了ZR/IAA、ZR/GA1,3,4,7、ABA/IAA和ABA/GA1,3,4,7比值.烯效唑处理增加了花芽形成百分率,加速了花芽分化的进程,缩短了花芽形成的延续时期,但对花芽生理孕育临界时期长短没有影响.烯效唑处理对花芽的节位数没有影响,但使叶芽节位数增加了1节.     

苹果花芽孕育机理的探讨

花芽孕育期,以环剥、多效唑＋环剥和ＧＡ３处理“红富士”苹果树,成花效应以多效唑＋环剥处理为最高（＋６８４％）。花芽孕育起动时,促花处理的短枝顶芽内ＩＡＡ、ＺＲ含量和ＩＡＡ／ＧＡｓ、ＺＲ／ＧＡｓ的比值均明显提高。在花芽孕育完成过程中,促花处理的短枝叶内淀粉含量、Ｃ／Ｎ比,芽内ＺＲ、ＩＡＡ含量和ＺＲ／ＧＡｓ明显提高,ＧＡｓ则明显下降。     

香港四照花花芽分化的形态学观察

采用石蜡切片技术和形态观察对香港四照花(Dendrobenthamia hongkongensis(Hemsl.)Hutch.)花芽分化过程中花芽的形态变化进行观测,研究花芽外部形态与花芽分化之间的关系。结果显示,香港四照花的花芽分化开始于7月上旬,到9月底完成,形态分化过程可分为8个时期:未分化期、花序原基分化期、小花原基分化期、花萼原基分化期、花瓣原基分化期、雄蕊原基分化期、雌蕊原基分化期、雌蕊雄蕊形成期。与之对应的外部形态变化为:混合芽闭合,混合芽基部膨大,新叶展开露出圆形花序,花柄初现,花序膨大,花序表面小花突起,花柄伸长至4~6 mm,花序表面小花轮廓明显。香港四照花花芽外部形态能直观地反映出内部结构变化,可根据花芽外部形态特征推测花芽分化状况。研究结果可为香港四照花花期调控和栽培管理提供科学依据。     

麝香石竹花芽离体发育的阶段控制

在离体条件下,利用不同的培养基对麝香石竹顶芽外植体的花芽发育进行了阶段控制的研究.结果表明,麝香石竹的顶芽外植体在MS+KT1.0mg/L+IAA1.0mg/L+蔗糖3.0%+琼脂0.8%的Ⅰ级培养基上能被诱导花芽发育的启动;然后,将已诱导花芽发育启动的顶芽外植体,转接到MS+KT1.0mg/L+IAA0.5mg/L+蔗糖1.5%+葡萄糖1.5%+琼脂0.8%的Ⅱ级培养基上能进行花芽的进一步发育形成花蕾,且能从一个花蕾继续分化发育重新产生2—3个花蕾;把花蕾再转接到改良的MS+BA2.0mg/L+NAA0.2mg/L+蔗糖1.5%+葡萄糖1.5%+琼脂0.8%的Ⅲ级培养基上,培养一周后花蕾的花瓣张开,花朵全部开放.不同麝香石竹品种,诱导花芽发育启动的效果不同,Scania品种诱导效果最好.花芽发育初期可溶性蛋白含量较高,但随着花芽发育的进程而迅速下降,不同花芽发育时期的过氧化物酶活性均强于营养器官.本文为花芽分化发育机理的研究创造了条件,也为鲜花生产探索了新路子.     

白桦花芽蛋白质双向电泳技术的建立

目的:初步建立白桦花芽蛋白质组研究的双向电泳(2-DE)技术,以提高其分辨率及重复性。方法:以白桦花芽为实验材料,对关键环节如样品处理、上样量和染色方法等进行一系列优化。结果:蛋白上样量为50～60μg、银染剂中采用0.16%的AgNO3染色12min,即可获得蛋白点的形态规则、稳定性高、重复性好的2-DE图谱。结论:建立了适合多糖、醌类等次生代谢物质含量较多的白桦花芽蛋白提取方法,为开展白桦发育生物学研究奠定了基础。     

外源激素在诱导风信子花被外植体不同部位细胞再生花芽中的作用

外源激素诱导风信子（Ｈｙａｃｉｎｔｈｕｓ ｏｒｉｅｎｔａｌｉｓＬ．）同一发育时期花被外植体不同部位细胞再生花芽的实验表明∶１． 诱导花被外植体细胞再生花芽,外源激素是必需的;２． 仅有细胞分裂素就可以诱导花芽再生,生长素并不是必需的;３． 花被外植体上的不同部位的细胞再生花芽时,需要不同浓度的外源激素． 单独加６－ＢＡＰ或玉米素２ ｍ ｇ／Ｌ可以诱导花被下部的细胞再生花芽;６－ＢＡＰ或玉米素２ ｍ ｇ／Ｌ和２,４－Ｄ ０．１ ｍ ｇ／Ｌ的组合有利于花被中部的细胞再生花芽;６－ＢＡＰ或玉米素２ ｍ ｇ／Ｌ和２,４－Ｄ １．０ ｍ ｇ／Ｌ的组合能促进花被上部的细胞分化花芽     

毛鹃‘紫萼’秋梢花芽发育的研究

本研究首次发现了毛鹃花芽分化过程中的一个特殊现象──秋季侧花芽伸长生长现象。并认为充足的光照,适宜的气温（２５°─２６℃）及充沛的降水伴随较高的空气相对湿度是导致这种花芽伸长生长的主要环境因子。也进一步证实了毛鹃是一类较喜阳生生境的灌木花卉。     

赤霉素对水涨龙眼花芽分化的效应

赤霉素100—300ppm11月下旬处理水涨龙眼,对花芽分化有一定的影响,但大小年间的反应存在差异,小年各处理间的花穗抽生率呈现出随浓度降低而提高的趋势,低浓度(100ppm)有明显的促花效应,而大年处理的花穗抽生率无明显差异。所有处理对花穗及夏、秋梢结果母枝的生长发育均无不良影响。     

The role of cytokinins in relation to flower-bud blasting in Iris cv. Ideal: Cytokinin determination by an improved enzyme-linked immunosorbent assay

The effect of dark and light treatment on endogenous cytokinins in internodes and buds of Iris was determined. Plant material was purified by chromatographic methods and cytokinins were assayed by an immunoassay.An indirect competitive enzyme immunoassay for the determination of zeatin- and isopentenyl-adenine cytokinins was developed. This assay, which is not dependent on the titre of the antibodies raised against zeatin riboside and isopentenyl-adenosine appeared to be specific, highly sensitive and more reproducible compared to a direct competitive enzyme immunoassay for cytokinins.Isopentenyl-adenosine was the most abundant cytokinin found, followed by zeatin: the latter counteracts bud blast when injected into dark-treated plants. Smaller amounts of isopentenyl-adenine and zeatin riboside were found. Results are in agreement with the hypothesis that deficiency of growth substances like cytokinins plays an important role in the occurrence of flower-bud blasting.A possible role for the major endogenous cytokinin, isopentenyl-adenosine, which earlier was found not to be effective in counteracting bud blast when injected into buds of dark-treated plants, is discussed.     

Growth factor combination for chondrogenic induction from human mesenchymal stem cell

During the last decade, many strategies for cartilage engineering have been emerging. Stem cell induction is one of the possible approaches for cartilage engineering. The mesenchymal stem cells (MSCs) with their pluripotency and availability have been demonstrated to be an attractive cell source. It needs the stimulation with cell growth factors to make the multipluripotent MSCs differentiate into chondrogenic lineage. We have shown particular patterns of in vitro chondrogenesis induction on human bone marrow MSCs (hBMSCs) by cycling the growth factors. The pellet cultures of hBMSCs were prepared for chondrogenic induction. Growth factors: TGF-beta3, BMP-6, and IGF-1 were used in combination for cell induction. Gene expression, histology, immunohistology, and real-time PCR methods were measured on days 21 after cell induction. As shown by histology and immunohistology, the induced cells have shown the feature of chondrocytes in their morphology and extracellular matrix in both inducing patterns of combination and cycling induction. Moreover, the real-time PCR assay has shown the expression of gene markers of chondrogenesis, collagen type II and aggrecan. This study has demonstrated that cartilage tissue can be created from bone marrow mesenchymal stem cells. Interestingly, the combined growth factors TGF-beta3 and BMP-6 or TGF-beta3 and IGF-1 were more effective for chondrogenesis induction as shown by the real-time PCR assay. The combination of these growth factors may be the important key for in vitro chondrogenesis induction.     

乳糖代替IPTG诱导重组人胸腺肽α1在大肠杆菌中的表达

研究以乳糖代替IPTG作为诱导剂诱导重组人胸腺肽α1表达的可行性,对乳糖诱导的时机、乳糖浓度、诱导持续时间以及其它诱导条件进行研究,确定了乳糖诱导的最佳条件。结果表明,乳糖能有效地诱导重组人胸腺肽α1的表达,并且目的蛋白的表达量略高于IPTG的诱导量。