小麦族几种近缘植物细胞在长期离体培养中的染色体变异

对小麦及其４种近缘属间禾草进行了长时间（０．５～５．７年,个别８．６年）的愈伤组织培养,在继代过程中染色体数目的变异在染色体倍性低的簇毛麦（Ｈａｙｎａｌｄｉａ ｖｉｌｌｏｓａ,２ｎ＝２ｘ＝１４）及新麦草（Ｐｓａｔｈｙｒｏｓｔａｃｈｙｓ ｊｕｎｃｅａ,２ｎ＝２ｘ＝１４）倾向于数目的增大;染色体倍性高的小麦（Ｔｒｉｔｉｃｕｎ ａｅｓｔｉｖｕｎ,２ｎ＝６ｘ＝４２）趋向于数目的减少;而倍性居中的羊草     

小麦及缺体小麦与黑麦杂种幼胚愈伤组织在长期继代中的染色体数量变异

对中国春及其６Ａ缺体与黑麦杂种幼胚愈伤组织在长期继代培养过程中愈伤组织的染色体数量进行了统计分析,结果表明：中国春×黑麦和６Ａ缺体×黑麦杂种幼胚愈伤组织在继代培养的前６０ｄ内细胞染色体数目分别稳定在２ｎ＝２８和２７;随着继代培养时间的延长,其染色体数量均发生变异主要表现为染色体数的减少;在第４２０ｄ至５４０ｄ培养期间两个组合愈伤组织丢失染色体的细胞比率明显增加,同时也发现了个别超出正常染色体数的细胞。第５４０ｄ后的愈伤组织染色体数量变异基本维持在这一水平。     

小麦及缺体小麦与黑麦杂种幼胚愈伤组织在长期继代中的染色体数…

对中国春及其６Ａ缺体与黑麦杂幼胚愈伤组织在长期继代培养过程中愈伤组织的染色体数量进行了统计分析,结果表明：中国春×黑麦和６Ａ缺体×黑麦杂种幼胚愈伤组织在继体培养的前６０ｄ内细胞染色体数目分别稳定在２ｎ＝２８和２７;随着继代培养时间的延长,其染色体数量均发生变异主要     

白Qian胚性愈伤组织长期继代培养中的分化能力及染色体稳定性 …

白Ｑｉａｎ（Ｐｉｃｅａ ｍｅｙｅｒｉ Ｒｅｈｄ．ｅｔ．Ｗｉｌｓ．）的胚性愈伤组织ＭＳ＋２,４－Ｄ１ｍｇ／Ｌ＋ＫＴ１ｍｇ／Ｌ的培养基上继代３年,增殖能力和分化潜力仍保持在原来的水平,没有明显降低的趋势。但随着继代时间的增长,胚性愈伤组织内有细胞的染色体数目发生了无规律的变化,而再生植株根尖细胞染色体数目比较稳定（２ｎ＝２８）。     

诱发小麦成熟胚愈伤组织及其再生植株抗盐性变异的研究

本研究以普通小麦成熟胚为起始材料,以平阳霉素(PYM)和正定霉素(ZDM)为诱变剂。发现不同基因型对药物的敏感性不同,其中对药物敏感的在含盐筛选培养基上的存活率高。在诱导培养基内添加一定量的诱变剂可以产生耐盐变异。这种抗性愈伤组织转入与筛选培养基含盐量相同的分化培养基,比较容易产生耐盐再生植株。其M_1、M_2代较亲本系表现株高降低,穗长变短、籽粒饱满度也差;M_1代的结实率仅有5.5%,M_2代恢复到40.9%。利用M_1代和亲本系实生苗叶片,进行脯氨酸含量测定。发现耐盐变异株在无盐的Hoagland溶液中,游离脯氨酸的含量超过亲本系,对盐胁迫不敏感,其耐受力强于对照,具有一定的抗盐稳定性。     

枣的花药离体培养和染色体倍性变异（简报）

附加不同浓度2,4-D、NAA、IBA和6-BA的MS培养基,离体培养二倍体金丝小枣（2n＝24）花药的结果表明,低温处理和生长调节剂可提高诱导率43．1％～49．6％。6-BA是分化小植株的决定因素,浓度1．0～2．0mg·L(-1),分化率为30．2％～44．7％。同一愈伤组织再生小植株染色体镜检为n、2n、3n、4n4类,倍性变异较大。     

银鹊树胚性愈伤组织继代培养过程中的细胞染色体数目变异

以银鹊树幼嫩的合子胚为外植体诱导胚性愈伤组织,胚性愈伤经增殖后转接到液体培养基中悬浮继代培养,对其多次继代培养的胚性愈伤细胞的染色体数目检测发现:多次继代培养后的胚性愈伤细胞染色体数正常的比例为48.28%(2n=30),部分细胞出现染色体数目2n=15~60的变异,其变异率高达51.72%,其中以亚二倍体变异为主(40.07%).结果表明,在体细胞胚胎诱导形成过程中,胚性愈伤组织细胞在染色体水平上发生部分变异,这可能是体胚形成过程中畸形胚产生的根本原因.     

陆地棉胚性愈伤组织的变异及高频胚胎发生

陆地棉（Ｇｏｓｓｙｐｉｕｍ ｈｉｒｓｕｔｕｍ Ｌ．）胚性愈伤组织在两年多的继代培养过程中,由淡绿或灰色疏松状转变成灰黄色致密团块状,胚胎发生能力经历了一个由低到高再到低的过程。培养两年半后,从中分离出３种不同的愈伤组织系。第一种可产生大量的胚状体;第二种可产生少量胚状体;而第三种失去了胚胎发生能力。第一种团块颗粒小,后两种团块颗粒大。通过选择培养第一种愈伤组织系,建立了３ 个陆地棉栽培品种的高频体细胞胚胎发生系。染色体观察显示：其变异频率随愈伤组织培养代数的增加而升高;３ 种不同的愈伤组织系中,二倍体细胞的频率大小依次为：第一种＞ 第二种＞ 第三种。此外,第一种含有较多的超二倍体细胞,而后两种含较多亚二倍体细胞     

多胺在离体培养的植物组织形态建成中的作用

本文概述了多胺在原生质体培养,外植体发生愈伤组织、不定根、不定芽、体细胞胚胎、花芽和小鳞茎等过程中的作用,并简述了它的作用机制。     

小麦幼胚培养高效成株系统的建立

研究探讨了不同的基因型、幼胚取材时期、4℃处理时间、盾片接种方式、分化及生根条件等对小麦幼胚培养再生成株特性的影响,并在此基础上建立了一套高效、可靠、重复性好的小麦组培再生系统。优化条件下,该系统从幼胚诱导致密愈伤组织的频率为89％,致密愈伤组织的分化频率诱导2周时为95％,培养近3个月时仍可达50％以上。此外还发现部分叶状结构当转至新鲜的分化培养基上时能够进一步发育成为芽苗。分化的芽苗在生根培养基上大多生成丛生苗。从基部切开后,每棵芽苗／分蘖均可独立成株。组培苗均可正常地开花结实。     

Isozyme Variability in Plants Regenerated from Calli of Cereus peruvianus (Cactaceae)

Morphological and isozyme variation was observed among plants regenerated from callus cultures of Cereus peruvianus. Different morphological types of shoots (68%) were observed in 4-year-old regenerated plants, while no distinct morphological variants were observed in plants grown from germinated seeds. Isozyme patterns of 633 plants regenerated from calli and of 261 plants grown from germinated seeds showed no variation in isocitrate dehydrogenase isozyme, and the differential sorbitol dehydrogenase, alcohol dehydrogenase, malate dehydrogenase, acid phosphatase, and peroxidase isozyme patterns observed in regenerated plants were attributed to nonallelic variation. Allelic variation was detected at three isoesterase loci. The proportion of polymorphic loci for both populations was 13.6% and the deviation from Hardy–Weinberg equilibrium for the Est-1 and Est-7 loci observed in somaclones was attributed to the manner in which the regenerant population was established. The high values for genetic identity among regenerant and seed-grown plant populations are in accordance with the low levels of interpopulation genetic divergence. In somaclones of C. peruvianus, morphological divergence was achieved within a short time but was not associated with any isozyme changes and also was not accompanied by biochemical genetic divergence.     

Variation of B Chromosome Associated with Tissue Culture in Wheat-rye Cross

In vitro variation of B chromosomes was studied by examining the callus cells derived from the immature embryos from a cross of Chinese Spring wheat （Triticum aestivum L.） and Fin 7416 rye （Secale cereale L.） carrying two B chromosomes. In 40-d-old callus cells, the numbers of B chromosomes ranged from one to four in 65.6% of the cells observed. The distribution of B chromosome numbers was associated with the ploidy levels of the normal chromosomes （A chromosomes）. The frequency of the cells with high numbers of B chromosomes （i.e., three or four B chromosomes） in the amphiploid cells with 56 A chromosomes was greater than those in the haploid cells with 28 A chromosomes. Although structural changes in the rye A chromosomes were observed, cytological observation and genomic in situ hybridization demonstrated that the rye B chromosomes were conserved in morphological appearance following tissue culture.     

重组SCIRR39多克隆抗体的制备及检测

目的：在大肠杆菌中表达大鼠脊髓损伤与修复蛋白39（SCIRR39）的C端抗原表位,并制备其多克隆抗体。方法：从大鼠脊髓全横断损伤脊髓cDNA中扩增1386bp的Scirr39基因编码框,亚克隆该基因编码蛋白C端359～461位氨基酸残基的DNA片段,插入表达载体,转化大肠杆菌BL21（DE3）,IPTG诱导表达,SDS-PAGE分析表达情况,切胶纯化目的蛋白;利用多克隆抗体制备技术,制备重组SCIRR39蛋白的多克隆抗体;用ELISA方法检测抗体效价,Western印迹检测抗体的特异性。结果：SCIRR39蛋白C端抗原表位与GST的融合蛋白在大肠杆菌中以可溶形式高表达,相对分子质量为37．9×103;获得抗SCIRR39蛋白C端抗原表位的兔抗血清,其效价达到1：104;Western印迹显示多克隆抗体能特异识别重组SCIRR39蛋白的C端抗原表位。结论：在原核系统中表达纯化了重组SCIRR39抗原表位蛋白,制备的重组蛋白多克隆抗体将用于检测SCIRR39在脊髓损伤过程中的表达变化。     

扶芳藤组织培养再生体系的建立

扶芳藤茎段比叶盘易产生不定芽;4种基因型中,圆瓣扶芳藤的不定芽再生频率远远高于其他3种;MS 6-BA 2.0mg·L-1是圆瓣扶芳藤不定芽诱导的最适培养基;低温处理10 d可显著提高不定芽的再生频率;暗培养对扶芳藤再生影响不大;扶芳藤诱导不定芽的最适pH范围在5.8～6.2之间;最适琼脂浓度为0.6%.     

Variation and Evolution in the Karyotype of Lycoris (Amaryllidaceae) V. Chromosomal Variation in L. sanguinea Maxim.

Abstract In 554 bulbs from 38 populations of Lycoris sanguinea , several chromosomal variations have been discovered. Most of the bulbs have a common karyotype consisting of 22 acrocentric ( A ) chromosomes. Though their frequencies are low, some rearranged chromosomes which are aberrant have been found. The aberrants are as follows: 1. Subtelocentrics ( ST ); 2. Telocentrics ( T' ); 3. Metacentrics ( M' ); 4. Very small acrocentrics (a); 5. Very small metacentrics (m); 6. Acentric fragments ( Ac ); and 7. Dicentrics ( Di ) chromosome. All can be easily suspected to be derived from A s. Some aberrations of the satellite chromosomes have been observed also. In addition, a new karyotype composed of 2n=32=31 A + 1 M' chromosomes has been found.     

小麦耐低磷相关性状的全基因组关联分析

通过对小麦耐低磷相关性状进行全基因组关联分析(GWAS,genome-wide association study),挖掘与小麦耐低磷性显著相关的单核苷酸多态性标记(SNP,single nucleotide polymorphism)位点及候选基因,为小麦耐低磷性状的遗传基础和分子机制研究提供理论参考。本试验以198份黄淮麦区小麦品种(系)为试验材料,设置低磷和正常磷营养液水培试验,利用小麦35K芯片对分布于小麦全基因组的11896个SNP,采用Q+K关联模型对小麦耐低磷性相关性状进行关联分析。结果表明,小麦耐低磷性状表现出广泛的表型变异,变异系数为15.65%~26.59%,多态性信息含量(PIC,polymorphic information content)为0.095~0.500。群体结构分析表明,试验所用自然群体可分为2个亚群,GWAS共检测到67个与小麦耐低磷相关性状显著关联的SNP位点(P≤0.001),这些位点分布在除3A、3B和3D以外的18条染色体上,单个SNP位点可解释5.826%~9.552%的表型变异。在这些显著位点中有4个SNP位点同时关联到了2个不同的耐低磷性状。对67个SNP位点进行发掘,筛选到7个可能与小麦耐低磷性有关的候选基因。TraesCS6A02G001000和TraesCS6A02G001100在锌指合成中有重要作用;TraesCS6A02G118100可能为低磷胁迫诱导基因;TraesCS5D02G536400、TraesCS1B02G154200和TraesCS5D02G536500与低磷胁迫相关酶类基因家族有关;TraesCS1D02G231200与植物DUF 538结构域蛋白有关,是植物胁迫相关调控蛋白候选基因。     

Genetic instability during embryogenic cloning of celery

Genetically marked tissues of celery (Apium graveolens) were employed to contrast genetic and chromosomal stability in serially bulk-transferred callus and regenerated plants. After six months in culture, 84% of the callus cells were karologically indistinguishable from normal, while the remainder exhibited chromosome loss and/or fusion. All of 50 clones derived from this tissue expressed the control phenotype with respect to heterozygous isozyme markers. Of 95 plants regenerated from the same tissue, 94 were phenotypically indistinguishable from the original explant donor, and cytogenetic analyses revealed the presence in 4.3% of an accessory chromosome, while the remainder were normal diploids. Analysis of the selfed progeny of these regenerated plants revealed the presence of a new recessive mutation causing abnormal leaf morphology at a frequency of 1.8%. Only one of 40 cells in 12-month-old callus tissue was karyologically indistinguishable from normal, the remainder consisting primarily of hypodiploids. The observation that all 50 clones were phenotypically heterozygous was statistically inconsistent with the hypothesis that hypodiploidy was associated with random complete chromosome loss. The culture had, at this point, lost the ability to regenerate. It is speculated that embryogenic cloning of celery may be suitable under certain circumstances for direct field establishment, but that levels of new genetic variation are sufficiently high to preclude its use for seed production.     

Shoot regeneration in long-term callus cultures derived from mature flowering plants of Cyclamen persicum Mill.

Summary In long-term callus cultures of Cyclamen persicum Mill. two types of tissue could be distinguished. One type featured a brown suberised outer layer and was poorly organogenic. The other type was yellowish in appearance and gave rise to many shoot buds. Both types co-existed on the same callus, the former prevailing. Selection for organogenic tissue resulted in cultures yielding approximately three times more petioles than random subcultures. Callus-derived shoots could be rooted and established in the greenhouse. The method allowed for the production of thousands of plants but the regenerants often showed deviant phenotypes and genotypes.Abbreviations BA 6-benzylaminopurine - BMP basal medium propagation - BMR basal medium rooting - DAPI 4,6-diamino-2-phenylindole - KIBA potassium salt of indole-3-butyric acid - kinetin 6-furfurylaminopurine - MS Murashige and Skoog - NAA 1-naphthaleneacetic acid     

Adventitous bud induction in vitro from juvenile leaves of Cupressus arizonica Green

Juvenile leaves of Cupressus arizonica Green (3–5 mm in length) from eight week old seedlings, were cultured on liquid medium supplemented with isopentenyladenine (2 mgl^-1). Buds formed from the explants after three weeks of culture, but further growth occurred only after transfer to half-strength medium without plant growth regulators. Histological analysis at different times of culture, showed an early mitotic activity within transfusion tissue, followed by dedifferentiation of epidermal and mesophyll parenchyma cells at the basal zone of the leaves. The differentiation of vascular nodules always preceded bud formation. The difficulty of conifers to root and grow beyond plantlet stage is discussed.