麝泌香盛期麝香腺超微结构和麝香分泌研究

雄麝特有的麝香腺,由于分泌行使化学通讯机能的信息素(Pheromone)麝香,结构特异。长期以来,国内外对麝香腺的结构和麝香分泌研究甚少,只有解剖学方面的简单描述,故对麝香分泌机理和泌香规律众说纷纭。我国最早(1958)进行过人工养麝和活体取香。随着养麝业的发展,近年对麝香腺进行了解剖、组织学(毕书增等,1980;冯文和等,1981;郑生武等,1984)和泌香机理研究(毕书增等,1980;李复东,1980;颜于宏等,1981),对麝香的分泌、形成与泌香规律有了进一步的认识,但缺乏全面系统的研究,特别在超微结构的研究方面尚属空白。     

Ultrastructure of the Vegetative Cells of Nostoc flagelliforme Prepared with High Pressure Freezing and Freeze Substitution Technique

The ultrastructure of the vegetative cells of Nostoc fiagelliforme Born. et Flah. was investigated with high pressure freezing and freeze substitution technique and compared with the results obtained by using conventional preparation methods. During the processes of chemical fixation, dehydration and embedding, the cell structures might be more artificially modified than that obtained from high pressure freezing and freeze substitution. With the present method, the sheath of N. fiageUiforme could be well-penetrated and no extra big space could exist between the cell and the sheath. The cell protoplasm rarely shrinked. Some fine structures of cell inclusions and unit membranes became visualized. Many bacteria were harbored in the sheath. In addition, the presence of big vacuoles in the cell of N. fiageUiforme as well as the presence of bacteria in the sheath shown in the present preparation for cyanobacteria has not been described so far in the literature.     

被孢霉γ-亚麻酸高产菌株选育

利用紫外线复合氯化锂诱变高山被孢霉SM96,筛选出一株高产γ-亚麻酸的菌株TM11,产量比出发菌株(25mg/L)提高了近3倍。对影响其多不饱和脂肪酸产生的因子Mg2+,VB6,营养盐溶液,磷源,碳源,氮源酵母膏进行了正交试验,选出TM11最佳的培养基配方:MgSO4·7H2O1.0g,VB6150mg/L,酵母膏6g/L,葡萄糖100g/L,营养盐溶液1mL/L,K2HPO42g/L。在上述最佳培养基中TM11的生物量达18.0213g/L,总脂达10.8128g/L,GLA量达668mg/L。     

枯盘斑多毛孢Pf-毒素组分的研究I.活性组分I的结构分析

以正丁醇:水:甲醇(4:2:1)作洗脱剂,通过硅胶H60型柱反复柱层析,将3种有致病活性的物质充分纯化,在-40℃下冷冻干燥后,它们为褐色深浅不一的蓬松状物质,且极易吸潮。活性组分I(Rf0.83)、活性组分II(Rf0.79)和活性组分III(Rf0.80)对马尾松切根幼苗和湿地松切根幼苗针叶都有致萎作用,通过质谱(MS)、核磁共振谱(1HNMR、)和红外光谱(IR)等分析手段确定出所分离的活性组分I的化学组成为C5H11O5N(M=165)。     

SCAR分子标记技术在香菇菌株鉴定上的应用研究

为了建立一套基于DNA分子标记技术快速鉴定香菇菌株的有效方法,本研究首先通过对生产上常用的14个香菇菌株进行RAPD多态性分析,从香菇菌株162中扩增获得了一个片段长为1166bp的特异RAPD标记XG1166,随之利用分子克隆技术将该特异RAPD标记成功转化为稳定的SCAR标记。用同样的方法,本研究又从另一香菇菌株申香10号中获得了一段长度为347bp的特异SCAR标记SX347。试验结果表明,利用本研究获得的香菇菌株162和申香10号的特异SCAR标记,能在一天时间内准确鉴定出香菇菌株162或申香10号菌株的真伪。由此可见,SCAR分子标记是一种快速、稳定、准确鉴定香菇菌株的新方法, 可应用于食用菌种质资源保护利用、品种分类与鉴定和假种辨别。     

链格孢菌原生质体的制备与限制性内切酶介导整合(REMI)转化的致病性诱变

以链格孢菌Alternariaalternata菌株NEW为供试菌株,研究了菌龄、酶系统、酶解时间、酶解温度及稳渗剂对链格孢菌原生质体制备的影响。结果表明,制备链格孢菌原生质体比较适宜的条件为PD液体培养基培养20h,以0.7mol/LNaCl为稳渗剂、1%LysingEnzyme、1%Drislase和1%Snailase3种酶溶液混合使用,30℃酶解3h。对原生质体进行了限制性内切酶介导整合(REMI)转化,筛选到了链格孢菌弱致病突变株NEW001,为致病相关基因的标记和克隆打下了基础。     

不同化学杂交剂(CHA)对小麦花药同工酶影响的研究

在小麦叶枕距±2cm时,喷施4种不同化学杂交剂（CHA）后,分别取小孢子处于不同发育阶段的花药,进行过氧化酶（POD）、淀粉酶（Amy）和酯酶（Est）等同工酶的分析。研究表明：在小孢子母细胞减数分裂期,处理2、3和4三种CHA对POD的A1、A2;B2、B4和B5,C1、C2和C3同工酶带的活性均有明显的抑制作用;处理5除去对A1和A2表现抑制外,对其他酶带的活性均有增强作用。在单枚早期,处理2和3的A、B和C区POD同工酶活性均明显低于对照;处理4和5上述各区POD同工酶活性却明显高于对照。在上述两个发育时期,处理2对Amy1区酶活性有增强作用,而处理3、4和5对该区酶活性却表现了专一性的抑制。各处理对Est同工酶A区和B区的酶活性主要表现为抑制。实验结果表明,不同的CHA均通过干扰花药的物质和能量代谢而导致雄性生理性不育。     

水稻抗白叶枯病基因Xa-4的PCR标记研究

根据与水稻抗白叶枯病基因Xa-4紧密连锁的分子标记M55的序列设计引物,通过对国际水稻研究所育成的抗白叶枯病近等基因系和基因累加系的叶片DNA、半粒种子提取物及Xa-4基因的杂合体DNA的PCR特异扩增,初步建立了Xa-4的PCR标记体系。进而用该标记体系对我国籼型杂交水稻常用的亲本材料进行分析,揭示出了Xa-4在这些材料中的分布情况。 Abstract　Based on the sequence of a DNA marker tightly linked to the rice bacterial blight（BB） resistance gene Xa-4, two primers were designated and synthesized to develop a PCR marker for the gene. Specific amplified polymorphism analysis was carried out with these primers on a set of BB resistance isogenic lines and pyramided lines developed by IRRI. Two PCR bands were revealed corresponding to lines with dominant Xa-4 and those with the recessive allele, respectively, regardless the lines pyramided with other resistance genes. A hybrid with heterozygous Xa-4 produced both of the two allele PCR pattern. Then, the PCR marker was used to survey a range of hybrid rice germplasm. The results of the germplasm survey will be useful in hybrid rice breeding programs aimed at exploiting Xa-4.