番茄SlWRKY31基因启动子的克隆与逆境应答模式分析

该研究以野生型番茄（Solanum lycopersicum）为材料,采用PCR技术克隆得到了番茄 SlWRKY31 基因起始密码子 ATG 上游启动子序列,并利用该启动子驱动 GUS基因在野生型番茄中表达,对获得的转基因番茄采用不同胁迫处理后进行GUS 染色和定量分析。结果表明：（1）序列分析显示,该启动子全长1 849 bp,含有多个与非生物胁迫和激素响应相关的顺式作用元件,主要包括热胁迫响应元件 HSE、干旱诱导响应元件 MBS、防卫和胁迫响应元件 TC rich repeats、创伤诱导响应元件 WUN motif、脱落酸（ABA）响应元件 ABRE 和水杨酸（SA）响应元件 TCA element。（2）实时荧光定量 PCR 结果显示,SlWRKY31 基因呈组成型表达模式,且在叶和果实中表达量较高,茎中较低;在NaCl、甘露醇、SA、ABA 和42 ℃ 高温的胁迫处理下,其表达量显著升高。（3）构建 SlWRKY31 启动子和 GUS 基因融合的植物表达载体,并通过农杆菌介导法将其转化野生型番茄,对获得的转基因番茄进行 GUS 组织化学染色分析结果显示,SlWRKY31 基因在番茄的各个组织（根、茎、叶、花、果实和种子）中均有表达,表明 SlWRKY31 启动子是组成型表达启动子。（4）对转基因番茄在不同胁迫处理后的 GUS 染色和定量分析显示,SlWRKY31 启动子显著受到NaCl、甘露醇、SA、ABA 和42 ℃ 高温的诱导表达,说明该启动子是一个可以响应多种逆境胁迫的诱导型启动子。     

垫状卷柏SpLEA1基因克隆及干旱胁迫下的表达分析

晚期胚胎发育丰富蛋白(late embryogenesis abundant,LEA),广泛存在于生物体内,与植物抗逆性密切相关,可在干旱胁迫下保护植物细胞,减少植物损伤。垫状卷柏(Selaginella pulvinata)是一种在干旱胁迫下生存能力极强的蕨类植物,具有很强的恢复能力。为探究垫状卷柏SpLEA1基因在耐旱植物中的分子机制与表达特征,该研究以高耐旱性植物垫状卷柏为实验材料,基于转录组测序结果,采用RT-PCR技术获得SpLEA1基因cDNA序列,采用HiTail-PCR技术获得启动子序列,利用生物信息学对序列进行了分析,并采用qRT-PCR技术分析了SpLEA1基因在干旱胁迫下的表达模式。结果表明:(1)垫状卷柏SpLEA1全长为476 bp,开放阅读框(ORF)为279 bp,共编码92个氨基酸,通过在线工具预测到蛋白分子量为9 491.46 Da, 等电点为5.45,蛋白结构预测分析表明该蛋白为亲水性蛋白,含有10个磷酸化位点,二级结构以α-螺旋和无规则卷曲为主。(2)预测到SpLEA1蛋白的保守结构域为Lea-5,来源于LEA1家族。基于系统发生树和遗传距离矩阵,发现垫状卷柏SpLEA1与来自鹰嘴豆(Cicer arietinum )和红车轴草(Trifolium pratense)的Lea-5蛋白同源性较高。(3)对启动子序列进行顺式作用元件的预测分析发现SpLEA1基因启动子含有5类激素响应元件和与干旱胁迫响应有关的功能元件。(4)在自然干旱处理下SpLEA1基因表达上调,并在12 h时达到峰值,在24 h干旱后进行复水处理,表达量显著下调。综上所述,SpLEA1基因在垫状卷柏中很可能参与了干旱胁迫响应机制的相关调控。该结果为进一步研究垫状卷柏SpLEA1基因在干旱胁迫下的功能及其表达调控机制提供了参考。     

番茄LeRma1基因的克隆与表达

以番茄‘哈大粉801’为试材,利用RT-PCR技术,克隆得到1个E3泛素蛋白连接酶基因LeRma1（GenBank登录号XM_004243764.1）。对LeRma1基因进行序列分析,并对LeRma1基因在番茄植株的不同部位以及在非生物胁迫（干旱、盐、碱、高温、低温）下的表达和生理特性进行研究,为培育和改良番茄品种提供理论依据。结果表明：（1）序列分析显示,LeRma1基因的cDNA全长序列729 bp,编码242个氨基酸,分子量为27.05 kD,理论pI 7.97;同源分析显示,番茄LeRma1蛋白与马铃薯的一致性最高（91%）。（2）半定量PCR检测表明, LeRma1基因在番茄根、茎、叶、花、果实中均有表达,且表达差异不明显。（3）干旱胁迫下,LeRma1基因在番茄叶片中优势表达,而在整个干旱过程中根部的LeRma1基因表达量变化不明显;抗旱相关基因LEA、 DREB2A、ABI3在干旱胁迫过程中,番茄叶片中均有表达,且其表达量呈上升趋势,而在根部DREB2A、ABI3基因基本没有检测到。（4）干旱胁迫过程中,番茄植株中丙二醛（MDA）含量呈显著升高趋势,质膜系统严重损伤,体内保护酶（SOD、POD、CAT）活性上升,且根部活性总体明显高于叶片。（5）在非生物逆境（盐、碱、高温、低温）胁迫过程中,LeRma1基因在番茄叶片和根部的表达几乎都有增强的趋势,且在叶片中均是胁迫3 h后诱导起始增强表达。研究认为,LeRma1基因是一个受干旱胁迫诱导增强表达的基因,且在叶片中优势表达,说明LeRma1基因对植物耐受干旱胁迫所起的作用存在一定的组织差异性,而且LeRma1基因可能参与番茄的干旱应答及信号转导过程,在番茄抵抗其他非生物胁迫中LeRma1基因也可能具有一定的作用。     

茶树CsBAP1基因的克隆与非生物胁迫和激素响应分析

该研究基于茶树转录组数据,从茶树‘龙井43’cDNA中克隆获得茶树CsBAP1基因,对其蛋白质序列特征和基因表达模式以及CsBAP1在茶树不同组织、不同激素处理及不同逆境胁迫下的表达水平进行荧光定量检测。结果显示：（1）克隆得到的茶树CsBAP1基因开放阅读框长度为543 bp,编码180个氨基酸;CsBAP1蛋白为亲水性蛋白,理论相对分子质量为19 398 Da,理论等电点为9.30,含有保守的Ca²⁺依赖性的C2结构域;茶树CsBAP1蛋白二级结构由8.89％的α 螺旋、7.78％的β 转角、35.56％的β 折叠和47.78％的随机卷曲组成;三级结构分析结果显示,CsBAP1包括螺旋和折叠结构,与二级结构吻合。（2）荧光定量分析结果显示, CsBAP1基因在茶树的花、花蕾、幼叶、老叶和成熟叶中均有表达,且在老叶中的表达量最高;外源施用ABA、IAA、MeJA、GA³以及SA均能够抑制茶树CsBAP1基因的表达;在高温（38 ℃）、低温（4 ℃）、干旱（200 g·L^-1 PEG）、高盐（200 mmol·L^-1 NaCl）胁迫下,CsBAP1的表达量均有所上调,且不同时间段的表达存在显著差异。该研究为进一步研究茶树CsBAP1基因的功能奠定了基础。     

藜麦CqSAP8基因克隆及其在非生物胁迫下的表达分析

该研究根据NCBI公布的藜麦胁迫相关蛋白(SAP)基因CqSAP8序列进行克隆,利用生物信息学分析CqSAP8蛋白序列、理化性质和结构特点,并采用qRT PCR方法检测CqSAP8基因表达的组织特异性及在非生物胁迫下的相对表达。结果表明：(1)藜麦CqSAP8基因CDS全长528 bp,编码175个氨基酸;预测CqSAP8蛋白分子量为18.73 kD,理论等电点为7.46,属于稳定的亲水性蛋白质;CqSAP8蛋白在N端和C端分别含有A20和AN1保守域,是SAP蛋白最典型的类型。(2)序列比对与进化分析显示,藜麦CqSAP8与甜菜BvSAP8、菠菜SoSAP8亲缘关系最近,序列相似性分别为89.66%和89.47%。(3)qRT PCR分析表明,藜麦CqSAP8基因在根、茎、叶、花和种子中均有表达,且在种子中表达量最高;CqSAP8基因在干旱和高温胁迫12 h表达量达到最大值,分别是对照的13.09和17.47倍,高盐和低温胁迫下的最大表达量均为对照的3.91倍,说明藜麦CqSAP8基因响应多种非生物胁迫应答;另外,藜麦CqSAP8的表达量在ABA胁迫下24 h急剧升高,推测CqSAP8基因在非生物胁迫前期的响应不依赖ABA。该研究为进一步研究CqSAP8基因功能及抗逆分子机制奠定了基础。     

核桃JrsHSP17.3基因克隆及温度胁迫响应模式分析

通过分析核桃（Juglans regia）转录组,鉴定获得核桃热激蛋白家族sHSP17.3基因的全长cDNA序列,命名为JrsHSP17.3。JrsHSP17.3基因开放读码框474 bp,编码产物含157个氨基酸,分子量为17.64 kD,理论等电点为5.35。为了研究该基因表达的组织特异性及温度响应模式,采用实时荧光定量PCR（qRT-PCR）方法,对高温和低温胁迫下JrsHSP17.3基因在根、茎、叶中的转录水平进行分析。结果显示,JrsHSP17.3基因在不同组织中均有表达;经高温（36 ℃～52 ℃）和低温（16 ℃～6 ℃）处理后,JrsHSP17.3基因均可被显著诱导,其中12 ℃胁迫1 h表达最高,为对照（非处理情况）的142.02倍。研究表明核桃JrsHSP17.3基因能够响应冷热温度胁迫,为进一步研究JrsHSP17.3基因的抗寒耐高温特性奠定基础。     

茶树TIFY基因家族鉴定及非生物胁迫下表达分析

TIFY基因家族在茶树激素信号转导及其逆境胁迫具有十分重要的作用。该文利用生物信息学方法对茶树基因组中的TIFY家族进行了鉴定,分析其理化性质、系统进化、基因结构、染色体定位、启动子区顺式作用元件、组织表达模式,并通过RT-qPCR对部分TIFY家族成员进行了非生物胁迫。结果表明:(1)茶树TIFY基因家族成员19个(CsTIFY1～CsTIFY19),分属于4个蛋白亚家族TIFY、JAZ、ZML 和 PPD,且不均匀地分布在8 条染色体上,按照进化关系及结构特点可分为 7 组,每组内具有相似的基因结构与保守基序组成。(2)CsTIFYs基因的启动子区具有多种包含激素和非生物胁迫响应的顺式作用元件,通过实时荧光定量(RT-qPCR)分析其家族成员对在茉莉酸甲酯、盐(20%氯化钠)、冷(4 ℃)以及干旱(20% PEG-6000)处理下反应强烈,部分基因在根与顶芽中有较高的表达量。由此推测,TIFY基因家族可能在茶树激素信号调控、胁迫响应、生长和发育等多方面发挥功能作用。     

葡萄CBF4基因生物信息学及其对低温和硅酸钾响应分析

为探究葡萄CBF4基因的结构和表达特征,该研究以葡萄为材料,对葡萄 CBF4基因进行生物信息学及低温和硅酸钾响应分析。结果表明:(1)CBF4蛋白定位在细胞核,有5个磷酸化位点和14个糖基化位点,无信号肽,是一个亲水的、脂溶性较差的膜外蛋白。二级结构以无规则卷曲为主,比例为56.88%。该蛋白包含一个AP2/EREBP结构域。(2)CBF4蛋白的多序列和系统进化分析表明酿酒葡萄与美洲葡萄的同源性最高、亲缘关系最近。(3)荧光定量 PCR 分析显示,低温胁迫后CBF4基因在葡萄叶片中表达水平上调,说明CBF4基因可能参与了葡萄叶片低温胁迫的响应。低温条件下,施加硅酸钾CBF4基因表达具有差异性,说明该基因在不同的葡萄组织中对硅酸钾的响应机制可能不同。以上结果为进一步研究葡萄CBF4基因的功能和机理奠定了基础。     

胡萝卜肉桂醇脱氢酶基因的克隆及其对非生物胁迫的响应

该实验采用RT PCR技术,从胡萝卜‘黑田五寸’中克隆获得了编码肉桂醇脱氢酶（Cinnamyl alcohol dehydrogenase, CAD）的基因DcCAD。DcCAD序列长1 074 bp,编码357个氨基酸。亲水/疏水性分析表明,DcCAD属于亲水性蛋白。系统进化分析显示,DcCAD与番茄CAD（XP_010314515.1）亲缘关系最近。荧光定量PCR结果显示,DcCAD基因在胡萝卜根、叶片和叶柄中的表达量差异显著,其相对表达量为叶片＞根＞叶柄。DcCAD基因对高温（38 ℃）、低温（4 ℃）、干旱（20% PEG）和盐（0.2 mol·L^-1 NaCl）胁迫均有响应,尤其对高温胁迫和低温胁迫响应明显,而且高温处理后1 h和低温处理后2 h表达量最高。研究推测,DcCAD基因对胡萝卜抗逆性具有一定的作用。     

蓖麻RcMsc2基因功能分析

G2/有丝分裂特异性细胞周期蛋白 2(G2/mitotic-specific cyclin-2,Msc2)作为高等植物应对逆境胁迫的关键调控蛋白,参与多个抗逆境胁迫的应答。为探究RcMsc2基因的功能,该研究从蓖麻叶片组织中成功克隆了RcMsc2,并利用生物信息学分析RcMsc2蛋白的结构和潜在功能,同时借助qRT-PCR方法分析RcMsc2基因的组织表达特性和非生物胁迫表达特性。结果表明:(1)RcMsc2基因位于蓖麻第5号染色体长臂,该基因的CDS(coding sequence)区是1 299 bp,编码432个氨基酸。(2)RcMsc2蛋白拥有细胞周期(cyclin)家族特征结构域,是一个不稳定酸性亲水蛋白,无跨膜域和信号肽,相对分子量为49.38 kD。(3)RcMsc2蛋白质的二级、三级结构以α-螺旋和无规则卷曲为主。(4)RcMsc2蛋白与麻风树和巴西橡胶树的CYCB2蛋白的序列同源性最高,且同被聚为Group Ⅱ。(5)35S-RcMsc2-GFP融合蛋白定位于细胞核。(6)RcMsc2基因在蓖麻的所有组织中均有表达且主要在根和茎中发挥作用; 非生物胁迫分析表明RcMsc2基因可以被脱落酸(abscisic acid, ABA)、盐、干旱和低温处理诱导表达,并且RcMsc2基因对低温胁迫的响应最敏感。综上表明,该研究较全面地分析了RcMsc2基因的结构特征、系统进化和表达模式,为揭示RcMsc2基因在蓖麻的生长发育和应答冷胁迫过程中的功能提供了理论参考。     

Presence of Rhizobium Etli bv . Phaseoli and Rhizobium Gallicum bv . Gallicum in Egyptian Soils

Seven bean rhizobial strains EBRI 2, 3, 21, 24, 26, 27 and 29 identified as Rhizobium etli, and EBRI 32 identified as Rhizobium gallicum, isolated from Egyptian soils and which nodulated Phaseolus vulgaris efficiently, were subjected to hybridization with a nifH probe in order to estimate the copy number of this gene. Seven strains (EBRI 2, 3, 21, 24, 26, 27 and 29) which were only able to nodulate Phaseolus vulgaris, contained three copies of the nifH gene, consistent with their identification as Rhizobium etli bv. phaseoli. Only one strain (EBRI 32) which nodulated both Phaseolus vulgaris and Leucaena leucocephala, had one copy of nifH gene. This confirmed the classification of this strain as Rhizobium gallicum bv. gallicum.     

Effects of MULTIFOLIATE-PINNA, AFILA, TENDRIL-LESS and UNIFOLIATA genes on leafblade architecture in Pisum sativum

In order to dissect the genetic regulation of leafblade morphogenesis, 16 genotypes of pea, constructed by combining the wild-type and mutant alleles of MFP, AF, TL and UNI genes, were quantitatively phenotyped. The morphological features of the three domains of leafblades of four genotypes, unknown earlier, were described. All the genotypes were found to differ in leafblade morphology. It was evident that MFP and TL functions acted as repressor of pinna ramification, in the distal domain. These functions, with and without interaction with UNI, also repressed the ramification of proximal pinnae in the absence of AF function. The expression of MFP and TL required UNI function. AF function was found to control leafblade architecture multifariously. The earlier identified role of AF as a repressor of UNI in the proximal domain was confirmed. Negative control of AF on the UNI-dependent pinna ramification in the distal domain was revealed. It was found that AF establishes a boundary between proximal and distal domains and activates formation of leaflet pinnae in the proximal domain.     

Characterisation of cell wall polysaccharides, arabinogalactans-proteins (AGPs) and phenolics of Cola nitida, Cola acuminata and Garcinia kola seeds

Many Cola plant species are endemic to West and Central Africa. Cola acuminata and Cola nitida are used as masticatory when fresh, while the dried nuts are used for beverages and pharmaceutical purposes in Europe and North America. Garcinia kola seeds, that serve as a substitute for the true kola nuts, are used in African traditional medicine for the treatment of various diseases, including colic, headache and liver cirrhosis. Seeds extracts of G. kola are also known for their anti-inflammatory, antimicrobial and antiviral properties. To gain information on the chemical properties of the kolas, we have isolated and analyzed cell wall polysaccharides, arabinogalactan-proteins and phenolic substances from the seeds of the three kola species. The sugar composition of cell wall material of C. acuminata, C. nitida and G. kola revealed that Gal (up to 30%), Ara, GalA and Glc as the predominant monosaccharides, representing approximately 90% by mol of the total hydrolysable sugar present in this material. In Ammonium oxalate cell wall fraction, GalA was found to be the major sugar present in all kola species. In the alkali-soluble fraction, there were significant differences in the level of Glc and Gal. The level of Glc was high in C. acuminata and C. nitida while the level of Gal and Xyl were high in C. nitida and G. cola. Isolation and quantification of arabinogalactan-proteins demonstrate that G. kola seeds contained four to eight times more of these proteoglycans than the seeds of the other two species. Finally, analysis of soluble phenolic substances shows that caffeine and catechin were largely represented in C. acumina and C. nitida seeds, with caffeine accounting for 50% of all soluble phenolics. These findings indicate that the three Kola seeds are highly enriched in pectins and proteoglycans and that C. acuminata and C. nitida can be used as a possible source of caffeine and catechin.     

Genome Analysis inNeurospora crassa;Cloning of Four Lociarginine-1(arg-1),methionine-6(met-6),unknown-7(un-7), andribosome production-1(rip-1) and Associated Chromosome Walking

We have cloned fourNeurospora crassagenes by complementation analysis. Cloned genes include thearginine-1(arg-1),methionine-6(met-6),unknown-7(un-7), andribosome production-1(rip-1) loci. Chromosome walks were initiated in ordered cosmid libraries from the cloned loci. A total of about 700 kb of theNeurosporagenome is covered in these walks.     

中国黑粉菌属和利罗黑粉菌属

黑粉菌属是Roussel 1806年建立的,全世界记载有三百余种,主要寄生于禾本科,是经济作物及牧草的重要致病菌·长期以来,对黑粉菌的邢子使用过各种名称,如厚垣孢子,冬孢子及黑粉孢子等.本文采用黑粉孢子以区别锈菌的冬孢子. 芳’(1979)在《中国真菌总汇》中列出黑粉菌属五十种及一个变型.作者经过显微结构和超显微结构的研究,承认其中二十九种为正确名称,八种及一变型为异名,顶黑粉菌(Ustilago acrearus Berk.)由于错拼而被废弃.埃地黑粉菌(Ustilago emodensis Berk.)被转移至利罗粉菌属(Liroa).另有十一种黑粉菌因缺少标本留待今后订正.自1979年以后,杨信东(1983)增加黑粉菌属二种我国新纪录,K.范基和郭林(1986)描述一新种,四种新纪录.在本文中,作者描述一新种:鸢尾蒜黑粉(Ustilago ixiolirii Guo L) ,孢子堆生在蒴果内,不开裂,黑色,粉末状.黑粉孢子球形,近球形,稀椭圆形, 12.5-21×10-21μm,黑褐色,壁厚1-1.Sμm,纹饰脑状.是迄今生在石蒜科植物上唯一黑粉菌的种,其它几种黑粉菌均属条黑粉菌属.本文增加七种我国新纪录.共计四十九种,寄生于六科四十四属植物,主要是禾本科和蓼科.这仅是黑粉菌属研究的初步报告,在全国范围内大量采集黑粉菌标本后,作者相信会有更多新种和我国新纪录被发现.利罗黑粉菌属(Liroa)是从黑粉菌属(Ustaligo)分出的,此属为单种属.     

The phylogenetic placement of Ostropales within Lecanoromycetes (Ascomycota) revisited

Results of molecular studies regarding the phylogenetic placement of the order Ostropales and related taxa within Lecanoromycetes were thus far inconclusive. Some analyses placed the order as sister to the rest of Lecanoromycetes, while others inferred a position nested within Lecanoromycetes. We assembled a data set of 101 species including sequences from nuLSU rDNA, mtSSU rDNA, and the nuclear protein-coding RPB1 for each species to examine the cause of incongruencies in previously published phylogenies. MP, minimum evolution, and Bayesian analyses were performed using the combined three-region data set and the single-gene data sets. The position of Ostropales nested in Lecanoromycetes is confirmed in all single-gene and concatenated analyses, and a placement as sister to the rest of Lecanoromycetes is significantly rejected using two independent methods of alternative topology testing. Acarosporales and related taxa (Acarosporaceae group) are basal in Lecanoromycetes. However, if the these basal taxa are excluded from the analyses, Ostropales appear to be sister to the rest of Lecanoromycetes, suggesting different ingroup rooting as the cause for deviating topologies in previously published phylogenies.     

Nomenclatural changes resulting from the transfer of tropical African Sarcostemma to Cynanchum ( Apocynaceae : Asclepiadoideae )

Summary  Four species of tropical African Sarcostemma are transferred to Cynanchum together with two subspecies of S. viminale. In addition, Sarcostemma mulanjense is reduced to subspecific rank under C. viminale.     

转Cry1Ac/1Ab基因棉花对异色瓢虫生长发育及其捕食功能的影响

【目的】为探究转Cry1Ac/1Ab基因棉花对异色瓢虫生长发育及其捕食功能的影响。【方法】以转Cry1Ac/1Ab基因棉与其亲本常规棉为实验材料,利用取食不同棉花品种叶片的棉铃虫饲喂异色瓢虫幼虫。【结果】与常规亲本棉相比,取食饲喂转基因棉花叶片的初孵棉铃虫幼虫的异色瓢虫幼虫从1龄发育至化蛹期时间延长0.77 d,但差异不显著;除1龄幼虫体重增加(0.0773 mg)外,其余各龄期幼虫体重均有所下降,但差异均不显著;异色瓢虫1、2、3、4龄幼虫对初孵棉铃虫捕食量均随棉铃虫密度的增加而增加,捕食功能反应均符合HollingⅡ圆盘方程。【结论】转Cry1Ac/1Ab基因棉花对异色瓢虫生长发育无显著影响,饲喂取食转Cry1Ac/1Ab基因棉花的棉铃虫对异色瓢虫捕食功能无显著差异。     

Prosthecium species with Stegonsporium anamorphs on Acer

Data from microscopic morphology, single-spore cultures, and DNA analyses of teleomorphs and anamorphs support the recognition of five species of Prosthecium with Stegonsporium anamorphs on Acer: P. acerinum sp. nov., the teleomorph of S. acerinum; P. acerophilum comb. nov., formerly known as Dictyoporthe acerophila; P. galeatum comb. nov., originally described as Massaria galeata; P. opalus sp. nov.; and P. pyriforme sp. nov., the teleomorph of S. pyriforme s. str. The morphology of both type specimens and freshly collected material was investigated. The teleomorphs have brown ellipsoidal ascospores with five distosepta and often a longitudinal distoseptum. The anamorphs of all species described here belong to Stegonsporium; their connection to the Prosthecium teleomorphs was demonstrated by morphology and DNA sequences of single spore cultures derived from both ascospores and conidia. The anamorphs and teleomorphs of all five Prosthecium species are described and illustrated by LM images, and a key to these species is provided. As perceived from this work, S. pyriforme is restricted to Europe and does not occur in North America, whereas S. acerinum is restricted to North America, not found in Europe. The host associations given in the literature are revised and evidence is provided that only A. opalus, A. pseudoplatanus, and A. saccharum are confirmed hosts of Prosthecium with Stegonsporium anamorphs. Molecular phylogenetic analyses of tef1, ITS rDNA, and partial nuLSU rDNA sequences confirm that the species with Stegonsporium anamorphs are closely related to P. ellipsosporum, the generic type species. Stilbospora macrosperma is confirmed as the anamorph of P. ellipsosporum by DNA data of single spore isolates obtained from both ascospores and conidia.