魔芋试管苗及种芋工厂化生产栽培技术研究

魔芋试管苗及种芋栽培试验结果表明 :试管苗采用土壤、蛭石 -珍珠岩和液体培养均可获得 2～ 2 0 g的种芋 ;种芋栽培以蛭石 -珍珠岩或透气性良好的土壤作基质最好 ,煤灰中有害物质对魔芋产生毒害作用     

魔芋试管芋营养液栽培生产原原种技术研究

在温室对魔芋试管芋立体多架层营养液栽培生产原原种技术进行了研究。以不同质量分数和比例的N、P、K、Ca、Mg等大量元素和MS培养基的微量元素配制成营养液,对魔芋试管芋进行立体多架层无土栽培试验,结果表明:生长状况和原原种的产量均以N∶P∶K∶Ca:Mg的比例为4∶1∶2.4∶0.2∶0.7的Ⅴ号营养液最高,光照强度以2000~6000 Lux为宜。该试验为魔芋营养液的配方研制及栽培管理技术提供了理论依据。     

魔芋微型试管芋(拟球茎)繁殖技术研究

在魔芋愈伤组织的基础上,研究了培养基组成、培养条件等因素对试管芋形成的影响。魔芋愈伤组织在添加6-BA3.0 mg.L-1、NAA0.5 mg.L-1、IBA0.5 mg.L-1、KT5.0 mg.L-1的MS培养基上,20 d后形成大量不定芽。待不定芽生长至约0.5~1 cm时,将温度控制在15~20℃之间,不定芽基部膨大,2个月后形成多达10个以上的微型种芋,种芋之间以愈伤组织相连。将微型种芋连同愈伤组织取出,栽培到适当的基质中,浇灌营养液使基质保持湿润,自然条件下萌发,出苗率在90%以上,叶片多达18片,当年每块微型种芋可形成5 g以上的多个子芋。     

魔芋良种繁育技术体系建设概况

概述了魔芋良种繁育技术体系建设的发展历程,重点介绍了魔芋种芋的三级繁育体系、根状茎两年速成法和(试管芋)二年速成良种繁育技术,为魔芋产业发展中成果的转化应用起到了引导作用.     

魔芋试管气生球茎的诱导研究

以谢君魔芋无菌试管苗为试材研究离体条件魔芋试管气生球茎的形成,利用正交试验设计对培养基及培养条件进行优化选择。结果表明叶片插入培养基7d后开始形成愈伤,并在复叶叶脉处形成1-2个气生球茎。培养基、培养温度、光照强度、碳源是魔芋试管气生球茎诱导的主要限制因子。改良MS培养基中添加NAA、Kt、碳源分别为0.5mg/L、0.5mg/L、4%S 4%M为最佳诱导培养基;最佳培养条件为温度28℃,光周期8/16,光照强度800lx。     

魔芋试管苗批量生产过程中外植体消毒灭菌技术研究

采用熏气法,可较为彻底地杀死魔芋球茎或根状茎的内生菌,再配合酒精、HgCl2等进行表面灭菌,可使初次接种污染率控制在10%以下,继代培养污染率控制在5%以下,从而建立魔芋试管苗的无菌繁殖体系,为试管苗的批量化生产提供了前提和技术保障。     

TDZ和KNO3对芋试管球茎诱导的影响

与浓度为5.0 mg·L-1的6-BA相比,浓度为0.2 mg·L-1的TDZ (thidiazuron)可以显著提高4个品种芋的单瓶试管球茎的个数.浓度为50 mmol·L-1的KNO3对芋试管球茎数量影响不大,但对鲜重有较大影响,单瓶试管球茎的鲜重提高幅度为12.9%.     

红香芋试管球茎膨大过程中主要碳水化合物含量以及淀粉合成相关酶活性的动态研究

为了探讨芋(Colocasia esculenta(L.)Schott)试管球茎膨大期间糖类物质积累特点,以红香芋无菌试管苗为材料,研究了高浓度蔗糖诱导条件下,红香芋试管球茎形成及膨大过程中主要碳水化合物的变化规律,以及与相关酶活性的关系。结果表明:(1)在红香芋试管球茎膨大过程中,果糖、葡萄糖和总可溶性糖含量均呈先升高后降低的变化趋势,果糖含量在诱导至第27天时达到最大值,而总可溶性糖和葡萄糖含量均在第34天达到峰值;蔗糖含量呈现先上升、后下降、再上升的变化趋势,在培养第48天时积累量达到最大值。(2)红香芋试管球茎总淀粉含量、直链和支链淀粉含量均随培养时间的延长而增加,至膨大后期总淀粉含量达到最大值,淀粉总含量约占干重的76%,并以支链淀粉含量为主。(3)解剖学观察发现,随着试管球茎的形成与膨大,贮藏组织中淀粉粒密度不断增大,至球茎膨大后期,淀粉粒布满薄壁细胞,并且处于比较稳定的水平。(4)诱导培养至第41天时,试管球茎的ADPG焦磷酸化酶和Q-酶活性均达到最大值,分别为1.22和2.39μmol·g~(-1)·min~(-1)。相关性分析发现,从茎基部开始膨大(20d)至ADPG焦磷酸化酶和Q-酶活性达峰值(41d)时,ADPG焦磷酸化酶活性与总淀粉含量、Q-酶活性与支链淀粉含量的相关系数分别为0.819和0.738,二者均呈极显著正相关。研究认为,淀粉的积累以及可溶性糖类含量的变化与红香芋试管球茎的膨大发育密切相关,并受到相关酶的调控。     

正交试验优化花魔芋组织培养条件

通过正交试验优化了魔芋愈伤组织生长及出芽的条件:以花魔芋切块为外植体,在MS(或1/2MS)+6-BA1.5+NAA0.5+IBA1.0+糖30%(pH6.2)的培养基上,暗培养15～20d后,光照12h/d,不仅愈伤组织生长旺盛,而且可以一步成苗,形成完整的植株,能够按要求分批生产试管苗。     

紫薯提取物对花叶芋试管苗生长的影响

实验以花叶芋无菌苗为材料,通过研究有机提取物种类,提取物浓度及提取物提取方式对花叶芋试管苗生长的影响,筛选出最适合花叶芋试管苗培养的天然有机提取物。实验结果表明：MS基本培养基中添加紫薯提取物时,花叶芋试管苗生长优于其他植物提取物;当紫薯提取物浓度为10％时,花叶芋试管苗长势最佳;比较紫薯上清液、沉淀物、混合液3种提取方式,紫薯混合液对花叶芋的生长最为有利。     

14-3-3 Proteins and regulation of cytoskeleton

The proteins of the 14-3-3 family are universal adapters participating in multiple processes running in the cell. We describe the structure, isoform composition, and distribution of 14-3-3 proteins in different tissues. Different elements of 14-3-3 structure important for dimer formation and recognition of protein targets are analyzed in detail. Special attention is paid to analysis of posttranslational modifications playing important roles in regulation of 14-3-3 function. The data of the literature concerning participation of 14-3-3 in regulation of intercellular contacts and different elements of cytoskeleton formed by microfilaments are analyzed. We also describe participation of 14-3-3 in regulation of small G-proteins and protein kinases important for proper functioning of cytoskeleton. The data on the interaction of 14-3-3 with different components of microtubules are presented, and the probable role of 14-3-3 in developing of certain neurodegenerative diseases is discussed. The data of the literature concerning the role of 14-3-3 in formation and normal functioning of intermediate filaments are also reviewed. It is concluded that due to its adapter properties 14-3-3 plays an important role in cytoskeleton regulation. The cytoskeletal proteins that are abundant in the cell might compete with the other protein targets of 14-3-3 and therefore can indirectly regulate many intracellular processes that are dependent on 14-3-3.     

S-腺苷甲硫氨酸的研究现状及应用前景

介绍了S-腺苷甲硫氨酸的制备方法及稳定性研究现状,并对其临床应用及市场前景进行了分析。     

利用支持向量机和马氏判别式预测人类polⅡ启动子

通过选取人类启动子与非启动子序列中不同的k-mer作为预测算法的基础特征,分别以三个区域（-249～-1;0～＋50;-30～＋30）的6-mer频数作为离散源参数构建离散增量,同时选取24个位点（-31～-21;-4-＋2;＋25-＋29）的3-mer频数作为位置打分函数的参数,分别利用支持向量机和马氏判别式为判别函数对启动子进行预测。用10折叠交叉检验来衡量两种算法的预测能力,预测结果成功率分别达到87．0％和87．9％。对于独立检验集,敏感性分别为62．7％和76．0％,特异性分别为77．5％和66.8％。     

Eimeria clethrionomysis sp. n., Eimeria gallatii sp. n., Eimeria pileata sp. n. and Eimeria marconii sp. n. from the red-backed vole Clethrionomys gapperi Vigors, from Pennsylvania.

Four new eimerian species are described from red-backed voles, Clethrionomys gapperi in Pennsylvania. Sporulated oocysts of Eimeria clethrionomyis sp. n. are ellipsoidal, 18.8 (16.5-21.5) x 14.9 (14.0-16.5) with elongate, ovoid sporocysts, 10.6 (9.5-12.0) x6.1 (5.5-7.0). The oocyst wall is smooth, with 2 layers, and thins, with terminal cap at one or both ends. Polar granules, dark Stieda body and sporocyst residuum are present. The oocyst residuum is absent. Sporulated oocysts of Eimeria gallatii sp. n. are ellipsoidal, 27.7 (21-32) x 19.3 (17-24) with ovoid sporocysts, 13.5 (12-15) x 8.8 (8-10). The oocyst wall is smooth, 2-layered, with a micropyle and thin wall at the end opposite the micropyle. Polar granules, Stieda body and sporocyst residuum are present. The oocyst residuum is atypical, of cobwebby material. Sporulated oocysts of Eimeria pileata sp. n. are subspherical to spherical, 25.2 (20.5-29.5) x 22.5 (19.5-25.5) with ellipsoidal sporocysts, 13.4(10.5-15.0) x 8.4 (7.5-9.5). The oocyst wall is rough, pitted, striated, 2-layered, with no micropyle. Polar granules, oocyst and sporocyst residuum, Stieda body and stiedal cap are present. Sporulated oocysts of Eimeria marconii sp. n. are ellipsoidal, 13.0 (10.5-15-0) x 10.6 (9.5-12.0) with elongate, ovoid sporocysts, 7.7 (7.0-8.5) x 4.2 (3.0-4.5). The oocyst wall is smooth, single-layered, with no micropyle. Polar granules, dark Stiedal body and sporocyst residuum are present. There is no oocyst residuum.     

The caudal bursa in the Heligmonellidae (Nematoda: Trichostrongylina). Characterization and hypothesis on its evolution

The different patterns of the caudal bursa of the Heligmonellidae (Nematoda) are redefined, taking into account the grouping of rays 2-6 and the sequence of origin of these rays from their common trunk. The type of symmetry of the caudal bursa is also redefined. The following patterns were observed and characterized: the basic patterns: types 2-3, 2-2-1, 1-3-1 and 1-4 and the intermediary patterns: type 2-3 tending to type 2-2-1, type 2-2-1 tending to type 1-3-1, type 1-3-1 tending to type 1-4 and type 2-2-1 tending to type 1-4. An evolutionary interpretation of the patterns is attempted and seems to follow the direction: 2-3 to 2-2-1 to 1-3-1 to 1-4. Seven atypical patterns are described. The caudal bursae were classified based on their symmetry: subsymmetrical, dissymmetrical and asymmetrical. Independently of the type of symmetry, the two latero-ventral lobes may have the same or different patterns. The type of symmetry, the ratio between the two latero-ventral lobes and a characteristic pattern were utilized to characterize the caudal bursae at the level of the genus and the subfamily. The combination of the right/left ratio and the type of symmetry gives heterogeneous results, with no real association between these characters. The most conspicuous asymmetries and dissymmetries were found among the Nippostrongylinae. The most frequent pattern in the Heligmonellidae is the basic type 2-2-1; types 1-3-1 and 1-4 are less frequent but are characteristic of several genera; type 1-4 is absent from the Heligmonellinae. Whatever the pattern, in the Heligmonellidae rays 4 and 5 are the last to diverge from the common trunk of rays 2-6.     

Eimeria lemuris n. sp., E. galago n. sp. and E. otolicni n. sp. from a Galago Galago senegalensis

SYNOPSIS. Three new species of Eimeria are described from the intestinal contents of a galago Galago senegalensis E. Geoff. imported into the Amsterdam Zoo from Africa. The oocysts of E. lemuris n.sp. are 44-57 by 38-47 μ and contain 4 sporocysts measuring 17-20 by 10.5–14 μ. The oocysts of E. galago n.sp. are 20-25 by 19-23 μ and contain 4 sporocysts measuring 9-12 by 6-9 μ. The oocysts of E. otolicni n.sp. are 23-31 by 22-28 μ and contain 4 sporocysts measuring 10-15 by 8-12 μ. A few Isospora resembling I. arctopitheci Rodhain, 1933 were seen.     

Ultrastructure of multiciliated collar cells in the pilidium larva of Lineus bilineatus (Nemertini)

Summary The ultrastructure of the apical plate of the free-swimming pilidium larva of Lineus bilineatus (Renier 1804) is described with particular reference to the multiciliated collar cells. In the multiciliary collar cells there are several, up to 12, cilia surrounded by a collar of about 20 microvilli extending from the cells' apical surface. The cilia have the typical 9+2 axoneme arrangement and are equipped with striated caudal rootlets extending from the basal bodies. No accessary centriole or rostral rootlet were observed. Microvilli surrounding the cilia are joined in a cylindrical manner by a mucus-like substance to form a collar. In comparison with many sensory receptor cells built on a collar cell plan the multiciliary collar cells of the pilidium larva apical plate are rather simple and unspecialized. In other pilidium larvae monociliated collar cells are found in the apical plate. The possible function and phylogenetic implications of multiciliated collar cells in Nemertini are briefly discussed.List of Abbreviations a axoneme - b basal body - c cilia or flagella - d desmosome - G Golgi apparatus - m mitochondria - mf microfilaments - mu mucus - mv microvilli - n nucleus - nt neurotubules - pm plasma membrane - r rootlet - ri ribosomes - v secretory vesicles     

The 14-3-3s

Multiple members of the 14-3-3 protein family have been found in all eukaryotes so far investigated, yet they are apparently absent from prokaryotes. The major native forms of 14-3-3s are homo- and hetero-dimers, the biological functions of which are to interact physically with specific client proteins and thereby effect a change in the client. As a result, 14-3-3s are involved in a vast array of processes such as the response to stress, cell-cycle control, and apoptosis, serving as adapters, activators, and repressors. There are currently 133 full-length sequences available in GenBank for this highly conserved protein family. A phylogenetic tree based on the conserved middle core region of the protein sequences shows that, in plants, the 14-3-3 family can be divided into two clearly defined groups. The core region encodes an amphipathic groove that binds the multitude of client proteins that have conserved 14-3-3-recognition sequences. The amino and carboxyl termini of 14-3-3 proteins are much more divergent than the core region and may interact with isoform-specific client proteins and/or confer specialized subcellular and tissue localization.     

Kinetic study of the thermal inactivation of cholinesterase enzymes immobilized in solid matrices

The thermal inactivation of immobilized cholinesterase enzymes (ChE) in solid matrices where the protein unfolding is blocked was studied, thus enabling investigation of the kinetics of the inactivation process directly from the native structure to the inactivated state. The thermal inactivation of butyrylcholinesterase (BChE), recombinant human acetylcholinesterase (rHuAChE), and eel acetylcholinesterase (AChE) enzymes was studied in dry films composed of poly(vinyl pyrollidone) (PVP), bovine serum albumin (BSA) and trehalose at 60 degrees -120 degrees C. The kinetics follows a bi-exponential decay equation representing a combination of fast and slow processes. The activation enthalpy DeltaH(#) and the activation entropy DeltaS(#) for each of the three enzymes have been evaluated. The values of DeltaH(#) for the fast process and for the slow process of BChE are 33+/-3, and 28+/-2 kcal/mol, respectively, and the values of DeltaS(#) are 0.84+/-0.04, and -18.2+/-0.5 cal/deg, respectively. The appropriate value of DeltaH(#) for rHuAChE is 26+/-2 Kcal/mol, for both processes and the values of DeltaS(#) are -17.6+/-0.9, and -23.0+/-0.9 cal/deg, respectively. Similarly, the values of DeltaH(#) for eelAChE are 30+/-3, 31+/-1 kcal/mol, and the values of DeltaS(#) are -6.7+/-0.5, -9.1+/-0.2 cal/deg respectively.     

Two new species of Eimeria from peacocks (Pavo cristatus) in Saudi Arabia

Fifteen fecal samples from peacocks (Pavo cristatus) in Saudi Arabia contained oocysts of Eimeria riyadhae n. sp. in two peacocks and oocysts of E. arabica n. sp. in one peacock. Sporulated oocysts of Eimeria riyadhae are ellipsoidal, 27-30.5 x 20.5-25 (28.8 +/- 1.3 x 22.4 +/- 1.6) micron, with a two-layered wall and bilobed polar body, but without a micropyle or residuum. The sporocysts are ovoid, 11-14.5 x 6.5-8 (13.2 +/- 1.2 x 7.2 +/- 0.6) micron with a thick, knob-like Stieda body and a residuum. Sporulated oocysts of Eimeria arabica are spheroidal, 17.5-21.5 x 17.5-21.5 (19.2 +/- 1.6 x 19.2 +/- 1.6) micron, with a two-layered wall and two refractile polar bodies, but without a micropyle or residuum. The sporocyts are elongate ovoid, 9.5-12 x 4-6.5 (11.2 +/- 0.9 x 5.5 +/- 0.88), with a small crescent-shaped Stieda body. The host bird belongs to the order Galliformis.