蝴蝶兰Phal.‘B’和Phalaenopsis.SogoYukidian‘V3’正反交后代花部性状分离表现

以蝴蝶兰Phal.‘B’和Phalaenopsis SogoYukidian‘V3’为亲本进行正反交,对杂交F_(1)代花部性状的分离表现进行统计分析。结果表明,正反交F_(1)代的花色花斑、唇部肉突颜色、唇部中裂片颜色分离类别基本一致;蝴蝶兰Phal.B的紫红色花斑可以遗传给后代,且作为父本更容易遗传;同时紫红色肉突与紫红色花斑的分布有一定的正向相关性,当花瓣上有紫红色花斑的,肉突颜色会显现紫红色,而花瓣上没有紫红色花斑的,肉突颜色则不会呈现紫红色,且会随着紫红色花斑面积的增加,紫红色肉突所占比例随之增加;而且紫红色花斑分布对中裂片的颜色有一定的影响,当花瓣上有紫红色花斑时,中裂片更易呈现红色,且Phal.B为父本时杂交后代中这种遗传影响尤甚。

SWOT Analysis of Phalaenopsis amabilis Industry in Zhangzhou City

Phalaenopsis amabilis industry in Zhangzhou City is analyzed by SWOT method,and the strengths,weaknesses,opportunities and threats of P.amabilis industry in the city are expounded.Furthermore,some suggestions for the development of P.amabilis industry in Zhangzhou City are put forward,in order to provide certain references for the development of P.amabilis industry.

基质与氮磷钾比例对蝴蝶兰(Phalaenopsis hybridium)生长发育的影响

试验于温室进行 ,利用正交试验及灰色关联度分析 (综合评价指数 ) ,研究了四种代用基质与施肥方法对蝴蝶兰生长发育的影响。结果表明 ,蕾期施肥和基质类型是影响蝴蝶兰开花数量的主要因子。灰色关联度最高 (Ri=0 .6 9337)的处理组合是水藓基质施肥 2 0 0(N ,mg/L) ,N P (P2 O5) K (K2 O ) =15 15 15,现蕾后以磷钾肥加微量元素处理 ;其次是锯末+沙 ,施肥 2 0 0 (N ,mg/L) ,N P K =2 0 10 10 ,现蕾前用磷钾肥加微肥处理 ;三是花生壳 +沙 ,施肥量 10 0 (mg/L) ,N P K =15 15 15。沙 +KD 1型高吸水树脂基质的Ri

蝴蝶兰Phalaenopsis ‘Frigdaas Oxford’和Phal.316杂交F_1代性状分离研究

以中小型-黄底红紫斑纹-蜡质花品种Phalaenopsis‘Frigdaas Oxford’（黄金豹）为母本，大花型-纯白无斑纹-纸质花品种Phal．316为父本进行常规杂交，对其F1代群体的性状分离进行研究。结果表明：F1代群体根据花部性状特点分为11个类群（Group 01-Group11），17个数量性状介于双亲之间或低于双亲或高于双亲，表现为中亲优势或正向超亲优势或负向优势；杂交后代在花色、斑纹、花朵质地、唇瓣须状物、株高等方面都发生了明显的性状分离，今后可以此为基础进行优良单株或株系的筛选，并为部分花部性状的定向育种提供参考。

蝴蝶兰Phalaenopsis ‘Frigdaas Oxford’和Phal. SH49正反交后代观赏性状遗传倾向研究

以花色、花斑类型、花朵质地、株型大小、花朵大小等为蝴蝶兰杂交育种的目标性状,对Phalaenopsis‘Frigdaas Oxford’和Phal.SH49及其正反交后代群体的观赏性状进行分析,研究育种目标性状在后代中的表现与分离。结果表明:正反交F_1代的分离规律和变化趋势基本一致,根据主要花部性状特点分为4个组群(G01~G04),杂交F_1代在9个数量性状的平均值表现均较中亲值明显降低,适合选育小株型或小花型后代个体;杂交F_1代在花底色、花斑类型、花朵材质等质量性状上变化丰富,不同花色的遗传能力与覆盖能力有所差别,存在较深花斑色覆盖遮挡住较浅花底色的花色表现,且出现了亲本没有的花斑变化,这些性状的分离特征和遗传倾向将给今后新个体或新单株的目标性状预测筛选提供更多参考和依据。

Transcription analysis of peloric mutants of Phalaenopsis orchids derived from tissue culture

Tissue culture has been widely used for mass propagation of Phalaenopsis. However, somaclonal variation occurred during micropropagation process posed a severe problem by affecting product quality. In this study, wild type and peloric flower buds of Phalaenopsis hybrids derived from flower stalk nodal culture were used for cDNA-RAPD and cDNA suppression subtractive hybridization analyses in order to study their genetic difference in terms of expressed sequence tags. A total of 209 ESTs from normal flower buds and 230 from mutants were sequenced. These ESTs sequences can be grouped into several functional categories involved in different cellular processes including metabolism, signal transduction, transcription, cell growth and division, protein synthesis, and protein localization, and into a subcat- egory of proteins with unknown function. Cymbidium mosaic virus transcript was surprisingly found expressed fre- quently in the peloric mutant of P. Little Mary. Real-time RT-PCR analysis on selected ESTs showed that in mutant flower buds, a bZIP transcription factor (TGA1a-like protein) was down-regulated, while up-regulated genes include auxin-regulated protein kinase, cyclophilin, and TCP-like genes. A retroelement clone was also preferentially expressed in the peloric mutant flowers. On the other hand, ESTs involved in DNA methylation, chromatin remodeling and post- transcriptional regulation, such as DNA methyltransferase, histone acetyltransferase, ERECTA, and DEAD/DEAH RNA helicase, were enriched in normal flower buds than the mutants. The enriched transcripts in the wild type indicate the down regulation of these transcripts in the mutants, and vice versa. The potential roles of the analyzed transcripts in the development of Phalaenopsis flowers are discussed.

蝴蝶兰黄花系品种Phalaenopsis‘Taipei Gold’和P.‘Sara Gold’杂交及其后代的遗传表现

以蝴蝶兰Phalaenopsis黄花系品种P.‘Taipei Gold’(2n=3x=57)作母本进行杂交育种有一个突出的问题是不育性障碍,为了克服这种障碍,多年来选择不同的父本进行杂交,终于发现采用P.‘Sara Gold’作父本进行杂交,收到蒴果1个,培育出杂交后代群体180株,其中有开花株99株。对杂交后代株高、冠幅、着花量、花径、花箭数、侧枝数及花色、唇瓣颜色和花瓣上的斑点进行观测记载。结果表明:杂交后代生长发育指标优于双亲的株数百分比:株高、冠幅、着花量、花径、侧枝数和花箭数分别占67.68%,86.87%,61.62%,24.24%,21.21%和26.26%;花瓣和唇瓣的颜色,基本遗传了双亲的特点,91%的后代花瓣颜色与双亲相似,74%的后代唇瓣颜色与双亲相似,90%的后代花瓣上出现了斑点。以P.‘Taipei Gold’作为母本成功杂交在国内首次报道,为蝴蝶兰黄花系杂交育种提供了实践依据。

小兰屿蝴蝶兰(Phalaenopsis equestris)NAC转录因子家族的全基因组序列鉴定及其进化分析

兰科植物具有多样的生物学特性和重要的商品特性。其中,小兰屿蝴蝶兰是第一个全基因测序的兰科植物,对其中重要基因家族的发掘是进行兰科植物基因组水平研究的重要环节。文章采用BLAST方法从小兰屿蝴蝶兰全基因组序列中筛选出NAC转录因子,并对这些转录因子进行进化分析、保守结构域和基因结构的分析。经过结构域确认,总共鉴定出86个含有典型的NAM结构域的NAC转录因子;其中,PEQU_23244和PEQU_40419两个基因的C-端各预测出1个跨膜区,属于MTFs(membrane-bound transcription factors)。多序列比对分析结果显示,其中16个基因的NAM结构域并不完整。将其余70个基因与拟南芥的NAC转录因子一起构建进化树,结果表明,这些基因可以分为group A和group B两大类,分别包含3个和12个亚家族。小兰屿蝴蝶兰group A的基因间蛋白序列和基因结构差异较大,而group B中的基因间则相对保守。对NAM亚家族基因的分析表明,该亚家族基因的NAM结构域高度保守,且与拟南芥CUC1、CUC2、CUC3高度同源。

蝴蝶兰黄色蜡质品种Phalaenopsis‘C27’与紫红纸质品种Phalaenopsis‘31’杂交F_1代性状分离研究

以纯黄色蜡质蝴蝶兰Phalaenopsis‘C27’为母本、紫红色纸质蝴蝶兰Phalaenopsis‘31’为父本,对其杂种后代植株性状和主要观赏性状的分离规律进行研究。结果表明,根据花部特征,可将F_1代分为7个组群,除Group 6花瓣为深紫红色隐条纹之外,其余6个组群均呈现花瓣底色条纹性状分离的显著特征。对F_1代观赏性状变异系数进行分析,花序长、花朵数、花梗长变异最大;其余性状介于双亲之间或低于双亲,表现为中亲优势或衰退。从植株性状变异系数分析,株高、植株冠幅、叶片数变异较大,其余性状变异都较小。本研究结果可为利用蜡质黄花的优点对纸质大红花观赏性状进行改良,选育特色蝴蝶兰优良单株和新品系奠定基础,并为蝴蝶兰花色育种及亲本选配提供指导。

Study on the rapid propagation of Phalaenopsis hybrid

This paper studied the rapid propagation technology of Phalaenopsis hybrid by using the peduncle buds as the explants, and screened out a kind of culture medium, which was simple, rapid, available and high rate of propagation.

Proteomics-Based Analysis of <i>Phalaenopsis amabilis</i>in Response toward <i>Cymbidium</i>Mosaic Virus and/or <i>Odontoglossum</i>Ringspot Virus Infection

Stress response at the protein level to viral infection in orchid plants has not been extensively investigated to date. To understand the proteomic basis of Phalaenopsis amabilis’s responses to Cymbidium Mosaic virus (CymMV), and/or Odontoglossum ring spot virus (ORSV), the total proteins were extracted from Phalaenopsis amabilis leaves infected with CymMV, ORSV, or both respectively. Differentially expressed proteins were identified by two-dimensional electrophoresis, and 27 of these proteins that had significant changes were further examined by mass spectrometry. Comparing CymMV-infected leaves with mock-inoculated ones, 2 proteins were significantly up-regulated, 9 were significantly down-regulated and 1 previously undetected protein was identified. 10 proteins were significantly up-regulated, 3 significantly down-regulated and 1 previously undetected protein was identified in ORSV-infected leaves. 6 proteins were significantly up-regulated and 9 significantly down-regulated proteins were found in co-infected leaves. These identified proteins are involved in disease resistance, stress response, transcriptional regulation, energy metabolism, protein modification and the previously unknown proteins were not involved with known protein pathways. Proteins significantly up-regulated were ATP sulfurylase, down-regulated proteins included glutamate decarboxylase isozyme 2, RNA polymerase alpha subunit and chloroplastic peptide deformylase 1A were proteins with similar alteration trend after all infection treatments. Significantly up-regulated were Thioredoxin H-type and down-regulated Cytosolic phosphoglycerate kinase I which were proteins that have been shown to be specifically regulated by the infection with CymMV. Significantly up-regulated were proteins like Rubisco large subunit, Triosephosphate isomerase, NADP-specific isocitrate dehydrogenase and Cinnamoyl CoA reductase CCR2 by the infection of ORSV. Protein regulation in coinfected leaves followed a pattern similar to that of any of the single virus infection results.

Enhancing Flower Stalk Emergence in Phalaenopsis by Red Light Supplementation

A key step in regulating the flowering of Phalaenopsis is to control the emergence of the flower stalk or spiking. Light quality is an important factor to regulate plant reproduction. We used either red or blue light emitting diodes (LEDs) to substitute for 10% photosynthetic photon flux emitted by white fluorescent tubes as the control (WC) at approximately 70 μmole·m-2·s-1 to examine the effects of enhanced red (WR) or blue (WB) light on spiking and the dawn-to-dusk fluctuations in the photosynthetic pigments and carbohydrates of Phalaenopsis aphrodite, which were grown in 7.5 cm diameter pots for six weeks. WR treatment significantly elevated the ratio of red to far-red light and the level of phytochrome photostationary state in concurrence with an increase in the spiking ratio and length, but had little effect on the concentrations of chlorophyll a and chlorophyll b in the leaf, levels of soluble sugars such as glucose, fructose, sucrose, and insoluble starch in the leaf and shortened stem, the locus of spiking, when compared to the other two treatments. Evidently, the spiking of Phalaenopsis is improved by dependent on the relative amount of active phytochrome expressed in the photostationary state.

The Development Situation and Countermeasures on Phalaenopsis aphrodite Industry in Guangdong

The Phalaenopsis aphrodite industry has the characteristics of high technology content,industrialization,modern management,organic combination of industry and strong radiation effect. On the basis of investigation,we expounded the current development situation of the P. aphrodite industry in Guangdong,analyzed the aspects of production elements and demand conditions based on the " diamond theory",and put forward suggestion and countermeasures for the development of the P. aphrodite industry.

基于转录组测序的蝴蝶兰低温胁迫响应MYB转录因子挖掘

为了探究MYB转录因子在抗冷型蝴蝶兰低温胁迫响应中的功能,从蝴蝶兰低温胁迫转录组文库中筛选出31条具有完整开放阅读框的MYB转录因子基因序列,对其蛋白质结构域、理化性质、系统进化、表达特性等进行分析。结果表明,有19条序列属于R2R3-MYB,其中所含R2氨基酸排列模式为W(T/S/I)X_(2)EDX_(2)LX_(7)GX_(3)WX_(2)(L/V/I)X_(3)(A/T/S)(G/S)LXR(C/T/S)GKSCRLRWXNY,R3氨基酸排列模式为(F/I/M/L)(S/T)X_(2)EX_(3)(I/V)(I/L/V)X(L/V)HX_(2)(L/W)G(N/T)(R/K)W(S/A)XIAX_(2)LPGRTDNE(I/V)KNXW-(N/R/H)(T/S/G);其余12条序列属于1R-MYB,R氨基酸排列模式为W(S/T)X(E/D)EHX_(2)FLX(A/G)X_(4)-(G/D)(R/K)G_(0~1)(A/D)W或W(S/T)X(E/K)(Q/E)(N/D)KXFE(R/K)AL(A/V)X_(3)(E/D)X(T/A)PXRW。这31条序列均具有Myb-DNA-binding结构域,平均相对分子质量为30 288.28,平均理论等电点为7.55,且都为疏水蛋白。蝴蝶兰MYB转录因子TRINITY_DN61754_c4_g1在抗冷品种大辣椒中的表达量于低温处理前后基本不变,但在不抗冷品种富乐夕阳中低温处理早期表达量就开始下降;TRINITY_DN74288_c0_g1在大辣椒中低温处理后48 h表达量显著增加,而在富乐夕阳中低温处理24 h后的表达量显著降低。结合其与小兰屿蝴蝶兰MYB转录因子的同源性分析及功能预测,推测这2个基因可能在蝴蝶兰低温胁迫响应过程发挥重要的作用。

蝴蝶兰‘大辣椒’花粉活力及柱头可授性探究

以蝴蝶兰‘大辣椒’的不同时期花朵为试验材料,利用TTC和联苯胺-过氧化氢法分别检测花粉活力和柱头的可授性,探索最佳的授粉时期,以期为杂交育种选择亲本提供参考依据。结果表明,随着开放时间的增长,蝴蝶兰花粉团颜色逐渐加深,体积变小,硬度增加;蝴蝶兰不同开放时期花粉最佳染色时间不同,花蕾期为24 h,其余时期为48 h;不同开放时期花粉的活力也有差异,小花蕾期>大花蕾期>开放1 d>开放5~15 d;小花蕾期柱头可授性较弱,大花蕾、开放1 d和开放5 d柱头可授性逐渐有所增强,开放10 d和开放15 d柱头可授性最强。

秋石斛胚性愈伤组织诱导及再生体系的建立

秋石斛(Phalaenopsis-hybrid Dendrobium)花姿优美、花色丰富,是热区重要观赏植物,具有极高的产业价值。本研究以秋石斛杂交种迷你(Den.Yaya Victoria)、水蜜桃(Den.Swirl)、三亚阳光(Den.Sonia Hiasakul)原球茎和无菌苗幼嫩茎段为外植体,探讨不同植物生长调节剂组合对不同品种秋石斛胚性愈伤诱导、不定芽分化及植株再生的影响。结果表明:在胚性愈伤组织诱导阶段,原球茎和生长2个月的幼苗茎段作为外植体诱导效果最佳,暗培养30 d即可获得胚性愈伤。3个品种的愈伤组织诱导最佳培养基是以MSD(MS+30 g/L葡萄糖+1 g/L花宝1号+8 g/L琼脂)为基本培养基,添加0.5 mg/L KT和0.2~0.5 mg/L 2,4-D。迷你、水蜜桃、三亚阳光的胚性愈伤诱导率最高分别为31.11%、22.78%和50%,其中迷你品种仅需15 d即可获得胚性愈伤。最佳胚性愈伤增殖培养基为MSD+0.5 mg/L IBA+0.5 mg/L KT,胚性愈伤状态保持良好且不发生分化,增殖倍数0.9。最佳分化培养基为1/2 MS+0.5 mg/L IBA+0.15 mg/L KT,在光照条件下,接种后的胚性愈伤组织能够快速诱导形成芽点,30 d内分化形成2~3片叶的幼苗,相同培养基中保持60 d能够自行生根获得完整再生苗。最佳生根培养基为1/2 MS+30 g/L蔗糖+0.5 mg/L NAA+8 g/L琼脂,生根率为100%,平均生根数5条,根长约1.3 cm。本研究所使用的胚性愈伤组织诱导、增殖和分化培养基具有一定的广谱性,可为后续秋石斛胚再生途径及分子育种研究奠定基础。

蝴蝶兰种质资源倍性鉴定及育性相关性研究

为探究蝴蝶兰种质资源倍性与育性的关系,本研究采用染色体计数法结合流式细胞术鉴定蝴蝶兰属33个品种(种或变种)的倍性水平,并通过完全双列杂交试验探究不同倍性蝴蝶兰种质资源的育性。染色体计数结果表明,二倍体和三倍体蝴蝶兰均有5个,均占15.15%;四倍体蝴蝶兰有10个,占30.30%;非整倍体蝴蝶兰有13个,占39.39%。蝴蝶兰不同品种之间染色体大小构成存在差异。流式细胞术检测结果表明,蝴蝶兰属25个品种(种或变种)的流式细胞术倍性估计结果与染色体计数结果相符。供试材料的流式直方图均呈现出3~4个峰,且循环值均大于0.1。杂交育性结果表明,作为亲本杂交的四倍体蝴蝶兰具有最高的坐果率和萌发率;在三倍体和非整倍体蝴蝶兰中,不同品种之间的育性差异较大,同一品种作为父本或母本杂交和自交后,其育性差异也较大。上述结果表明,大多数蝴蝶兰杂交品种的倍性为多倍体或非整倍体,蝴蝶兰的育性与其倍性水平和染色体大小构成相关;流式细胞术的倍性估计适用于蝴蝶兰种内以及含有小而均匀染色体的杂交品种;供试蝴蝶兰叶片均存在内多倍体化且不同倍性蝴蝶兰叶片的内多倍体化模式存在显著差异。本研究为蝴蝶兰种质资源鉴定、亲本选配、遗传改良以及多倍体育种提供了参考依据。

外源BRs对不同品种蝴蝶兰开花性状的影响

蝴蝶兰开花性状影响其商品价值,以蝴蝶兰为材料,试验不同浓度的外源油菜素内酯(BRs)处理对3个品种的蝴蝶兰花葶数量、花葶长、花朵数、花朵直径、花期长度等开花性状的影响。结果表明,外源BRs处理对蝴蝶兰花葶数并无显著影响,但能使蝴蝶兰花葶提前发育,促进花葶伸长,增加花葶直径,并且BRs能使花朵提前开放,提升花朵数与花朵直径,延长开花花期。不同浓度的BRs处理,可以提升蝴蝶兰开花品质,不同处理浓度之间对不同品种蝴蝶兰开花性状的影响有显著差异。

辐射诱变小兰屿蝴蝶兰叶片生长与表型差异品种间ISSR分析

使用60Co-γ射线对小兰屿蝴蝶兰进行辐射处理,分别对单唇瓣、三唇瓣品种采用15 Gy和20 Gy剂量的处理,采用简单重复序列区间扩增多态(ISSR)分子标记技术对经辐射处理的小兰屿蝴蝶兰材料进行遗传多样性和亲缘关系分析.筛选出8条引物,共扩增出89条清晰的谱带,其中72条表现出多态性,多态比例为80.9%.单唇瓣品种之间遗传相似范围在0.54~0.97,三唇瓣品种之间遗传相似范围在0.54~0.91,说明辐射突变品种之间有丰富的遗传多态性.单唇瓣小兰屿蝴蝶兰经过辐射后,在遗传距离L=0.65处可分为4组,三唇瓣小兰屿蝴蝶兰经过辐射后,在遗传距离L=0.72处可分为7组.观察生长表型发现:经辐射处理的小兰屿蝴蝶兰出现生长快速表型,部分经辐射处理的单唇瓣株系生长率比对照组更高,而经辐射处理的三唇瓣株系生长率普遍比对照组高.非加权组平均法(UPGMA)聚类分析表明:小兰屿蝴蝶兰经过辐射诱变后有不同程度的突变,突变程度最大的品种在遗传距离图谱上自成一支.以上结果为培育优质蝴蝶兰品种奠定了材料基础.

低温胁迫下小兰屿蝴蝶兰叶片转录组分析

本文以小兰屿蝴蝶兰为试验材料,设置了低温胁迫组(4℃)和对照组(24℃)进行转录组测序,通过采用GO数据库、KEGG数据库比对,分析了差异基因的功能以及调控通路。结果显示:低温胁迫下共获得2865个差异基因,其中有471个为上调基因,有2394个为下调基因。GO富集分析可以将差异基因分为生物过程、细胞组分、分子功能三大类;KEGG通路分析结果得知,差异基因注释到125个不同代谢通路中,其中较多的差异基因富集于代谢过程、次级代谢物的生物合成、核糖体的代谢通路中。