Flower-inducing and -inhibiting activities of Phloem Exudate from Cotyledons of Pharbitis Seedlings

The flower-inducing and -inhibiting activities of phloem exudate (PE) prepared from cotyledons of Pharbitis seedlings were examined, using apex cultures in vitro from Pharbitis as a bioassay system.The PE was prepared from photoperiodically-induced cotyledons (SD-PE). The SD-PE was subjected to the following fractionations: When the SD-PE was extracted with CHCl₃ and then ethyl acetate, the inducing activity was located in the final aqueous fraction. The activity was localized in the diffusate when the aqueous fraction was dialyzed (molecular weight cut off was 10,000). The diffusate was fractionated by ion exchange chromatography, and flower-inducing activity was found in the fraction adsorbed onto anion exchange resin. When the fraction was applied to a Sep-Pak C18 cartridge, the activity eluted with 25% MeOH. As a result of the above fractionation, activity was increased about 30-fold.The nature of the flower-inhibiting activity of the PE taken from cotyledons exposed to continuous-light conditions was examined (CL-PE). The inhibiting activity was decreased as the cotyledons were exposed to longer dark periods; it appeared to be heat-stable. The CL-PE also inhibited flowering in Lemna. The CL-PE was subjected to the following fractionations: When the CL-PE was extracted with CHCl₃ and ethyl acetate, activity was located in the final aqueous fraction. Activity was localized in the diffusate when the aqueous fraction was dialyzed (molecular weight cut off was 10,000). When the diffusate was fractionated by ion exchange chromatography, the activity was found in the flow-through fraction. When the fraction was applied to a hydroxyapatite cartridge, the activity eluted with 25 mM sodium phosphate buffer. When the fraction was re-dialyzed (molecular weight cut off was 1,000), the diffusate contained the activity. As a result of the above fractionation, activity was increased about 10-fold.     

濒危植物秦岭冷杉补光育苗技术研究

秦岭冷杉种子生活力差、成苗率低(2.2%)是制约种群恢复的薄弱环节。通过对播种后苗期2年连续补光处理,幼苗表现出良好的生长效应,苗高10.5 cm(对照为7.3 cm),地径4.5 mm(对照为2.7 mm),保存率88.6%(对照66.4%),延长了幼苗生长期,增加了苗木生物量积累,加快了苗木培育进程。     

Fe3+络合萃取法从野葛根中分离葛根素

利用Fe3 + 能够和葛根素生成可溶性络合物的性质建立了一种从中药野葛根中萃取葛根素的新型分离方法。以甲醇冷浸从野葛根中提取葛根总黄酮 ,将其进行水解、中和 ,再给水解葛根总黄酮中加入FeCl3 使葛根素与Fe3 + 络合溶解 ,过滤除去其它不溶性物质 ,用盐酸解聚Fe3 + 葛根素络合物 ,则得葛根素粗品 ,将其重结晶可得葛根素。同时 ,利用分光光度法确定了Fe3 + 葛根素络合物解聚的最佳酸度。利用TLC标准品对照、IR和分光光度法对产品进行了定性和定量分析。该方法从葛根中提取葛根素收率为 1 2 % ,纯度为 96 5 % ,具有操作简便、工艺流程简单 ,容易实现工业化的优点。     

海洋创伤弧菌反式翻译系统关键因子SmpB基因的克隆及原核表达

创伤弧菌(Vibrio vulnificus)是一种重要的"人鱼共患病"病原菌。通过克隆创伤弧菌反式翻译系统核心因子小蛋白B(Small molecular protein B,SmpB)基因,构建携带目的基因的原核表达质粒,为后续研究SmpB蛋白的互作网络、SmpB蛋白与创伤弧菌致病性之间的关系并以此开发新型的抑菌靶标奠定基础。使用LiCl沉淀法提取创伤弧菌基因组DNA,以它为模板,PCR扩增目的基因,并构建到pET-28a原核表达载体上测序鉴定后对SmpB序列进行生物信息学分析,将正确的重组质粒转化E.coli BL21(DE3),IPTG诱导表达,SDS-PAGE凝胶电泳鉴定。结果表明使用LiCl沉淀法成功提取到高质量创伤弧菌基因组DNA,以其为模板,扩增到smpB基因,并成功构建pET-28a原核表达重组质粒,测序鉴定正确;smpB基因全长为486 bp,编码161个氨基酸,分子量为18.41 kD,理论等电点为10.28,不稳定系数为35.02,总平均亲水性为-0.635,SmpB蛋白整体表现为稳定亲水性蛋白。生物信息学分析显示其高级结构核心部分为5个β折叠组成的桶状结构,外围由3个α螺旋组成,SmpB C-端亦为α螺旋。诱导表达的重组融合蛋白相对分子质量大小在25.0 kD附近,显示在E.coli中成功表达了SmpB蛋白。     

白腐菌紫外诱变选育高产漆酶突变株及其产酶条件研究

以白腐菌为出发菌株,利用紫外线(UV)进行诱变,筛选高产漆酶突变菌株。通过测定致死率绘制出发菌株的致死曲线,采用PDA-RBBR平板变色法进行初筛,ABTS检测酶活对突变株进行摇瓶复筛。结果表明:利用15 w紫外灯在照射距离为30 cm,照射时间为120 s,致死率为72.1%的条件下进行诱变处理,获得一株高产菌株,其酶活提高79.54%,经过5代传代培养,未见酶活下降,具有较好的遗传稳定性,进一步研究了初始pH值,接种量和培养基装液量等对诱变菌株产酶的影响,结果表明在最佳的培养条件pH值6.0,15%的装液量于28℃下,酶活达214.9 U/L。     

人正常腺上皮组织中MUC6基因的表达

应用免疫组织化学和原位杂交方法检测人正常腺上皮中MUC6基因的表达,揭示MUC6基因在正常人腺上皮组织中的分布异质性及其特点.结果显示MUC6基因编码的核心蛋白及其mRNA主要分布于正常胃粘膜胃腺的基底部,上皮细胞无MUC6基因表达,呈细颗粒状,位于细胞核周,胃底、胃窦的表达无区别;十二指肠绒毛上皮内的表达呈弥漫性,均质状,杯状和柱状细胞的表达类似,杯状细胞的粘液滴内未测得MUC6基因产物;空肠、结肠组织中无MUC6基因的表达;胆囊上皮组织内有强阳性MUC6核心蛋白的表达,而宫颈上皮中表达较弱.实验提示MUC6基因的表达存在异质性及器官特异性.     

甾体化合物RSA的11β-羟基化反应

原生质体在甾体中的应用起始于Ｄｌｕｇｏｎｓｋｉ在 1984年采用Ｃｕｎｎｉｎｇｈａｍｅｌｌａｅｌｅｇａｎｓ转化可的松龙 ( 17α ,2 1 二羟基孕甾 4 烯 3 ,2 0 二酮 )和Ｈｙｐｈｏｄｅｒｍａｒｏｓｅｕｍ转化 6α 氟 可的松龙 16,17 醋酸酯 ( 6α Ｆｌｕ 17α ,2 1 二羟基孕甾 4 烯 3 ,2 0 二酮 16,17 醋酸酯 ) ,发现原生质体具有甾体转化能力[1 ,2 ] 。Ｓｅｄｌａｃｚｅｋ进一步采用等重的原生质体和菌丝体进行比较 ,原生质体的羟基化能力较后者提高了 3倍 ,表现出很高的转化能力[3] ,从而引起人们的关注。随后展开了有关原生质…     

云南丽江山慈菇遗传多样性的DALP分析

采用DALP (Direct amplification of length polymorphism) 分子标记技术, 对产自云南的药用植物丽江山慈菇Iphigenia indica (L.) Kunth的9个居群进行DNA指纹检测。筛选出5个引物组合, 扩增共产生131条DNA片段, 其中104 条谱带具有遗传多态性, 约占79 39%, 平均每组引物扩增所得多态条带为20 8, 9个居群平均多态百分率为42 21%。9个居群平均观察等位基因数Na为1 4224, 总Na为1 7939; 平均有效等位基因数Ne 为1 3141, 总Ne 为1 4810; 平均遗传多样性指数H为0 1745, 总H为0 2831; 平均Shannon 多样性指数I 为0 2527, 总I为0 4231; 总基因多样性Ht为0 2831, 居群内多样性Hs 为0 1745, 居群间基因分化系数Gst为0 3834, 即丽江山慈菇有61 66%的遗传变异来自居群内, 38 34%来自居群间, 居群间存在较高水平的遗传分化。滇西北居群的遗传多样性明显高于滇中居群的遗传多样性, 这与滇中地区丽江山慈菇野生资源被大规模挖掘有着直接的关系。     

Cadaveric study of the arterial anatomy of the upper lip

Arterial distribution of the upper lip was investigated in this study. The location, course, length, and diameter of the superior labial artery and its alar and septal branches were determined on 14 preserved cadaver heads. Another cadaver head was used to show the arterial tree by the colored silicone injection technique. The superior labial artery was the main artery of the upper lip and always originated from the facial artery. The superior labial artery was 45.4 mm in length, with a range from 29 to 85 mm. The mean distance of the origin of the superior labial artery from the labial commissura was 12.1 mm. The superior labial artery was 1.3 mm in external diameter at its origin. The mean distance of origin of the superior labial artery from the lower border of the mandible was 46.4 mm. The alar division of the superior labial artery was mostly found as a single branch (82 percent). Its mean length was 14.8 mm and the mean diameter at the origin was 0.5 mm. The distance between the origins of the superior labial artery and the septal branch was 33.3 mm. The septal branch was single in most of the cases (90 percent). The mean length of the septal branch was 18.0 mm and the diameter at its origin was 0.9 mm. After all dissections, it was concluded that the arterial distribution of the upper lip was not constant. The superior labial artery can occur in different locations unilaterally and bilaterally, with the branches showing variability.     

Phospholipase activities in subcellular fractions of human platelets.

A homogenate of human platelets was fractionated by zonal ultracentrifugation into membranes, various granules and mitochondria. The membrane fraction was composed of two populations. The first, which represented 75% of the proteins, was rich in plasma membranes; the second, which represented the remaining 25%, was rich in microsomal membranes. Lysophospholipase was essentially localised in the cytosol. Phospholipase A1 which was only weakly bound to membranes, was mostly found in the soluble fraction (75%); the remainder was located in the plasma membranes and the mitochondria. Two-thirds of the phospholipase A2 was found in the particulate fractions.     

Selective inhibition by ionophore A23187 of the enzyme isomerization in the catalytic cycle of sarcoplasmic reticulum Ca2+-ATPase

The effect of a lipophilic antibiotic, ionophore A23187, on the purified Ca2+-ATPase from sarcoplasmic reticulum was investigated. When the enzyme was pretreated with A23187 in the presence and absence of Ca2+, the Ca2+-dependent ATPase activity was inhibited almost completely, but the activity of the contaminating Mg2+-ATPase was unaffected. The steady state level of the phosphoenzyme (EP) from ATP or Pi was not substantially altered. When the pretreatment was performed in the presence of Ca2+, EP formation from ATP was only slightly retarded, but EP decomposition was strongly inhibited. Under these conditions, the accumulated EP was ADP-sensitive. EP formation from Pi after chelating of Ca2+ was quite slow, whereas EP once formed was in rapid equilibrium with Pi of the medium. On the other hand, when the pretreatment was performed in the absence of Ca2+, EP formation from ATP was extremely slow, but EP once formed was in rapid dynamic equilibrium with ATP of the medium. EP formation from Pi was very fast, and this EP was in rapid equilibrium with Pi of the medium. These results demonstrate that A23187 selectively inhibits isomerization of the enzyme between the high Ca2+-affinity form and the low Ca2+-affinity form in the catalytic cycle, whether or not the enzyme is phosphorylated. This suggests that interactions between the enzyme protein and the surrounding lipids could play a crucial role in this isomerization.     

BrdU抗血清制备和应用的研究——Ⅰ.高度特异的BrdU抗血清的制备与特性

半抗原BrU通过与BSA偶联制备了完全抗原,经过光吸收、SDS聚丙烯酰胺凝胶电泳和琼脂糖凝胶电泳的测定表明,核苷-蛋白质复合物符合制备的要求,每个BSA上估计大约平均有10.3个BrU。用常规免疫的方法获得兔抗BrdU的抗血清,与BrU-EA的双向扩散效价高达32。抗血清稀释128万倍时仍可见明显的ELISA阳性反应。与以前所报道的BrdU抗血清不同,该抗血清具有高水平的识别能力,已达到BrdU单克隆抗体的识别水平,无须纯化即可用于染色体及核酸的研究。     

生长激素释放激素和人血清白蛋白融合蛋白的克隆表达

目的:通过与人血清白蛋白(HSA)融合,延长生长激素释放激素(GHRH)在体内的半衰期。方法:根据毕赤酵母偏爱密码子重新设计GHRH的核酸序列,并通过化学合成和重叠PCR法将GHRH的N端与HSA的C端通过一个11肽的接头连接,获得GHRH和HSA融合的全长基因序列。构建pPIC9-HSA-GHRH表达载体,电击转化毕赤酵母GS115感受态细胞,通过表型筛选和诱导表达实验得到蛋白表达工程菌,对表达产物进行分离纯化和生物学活性分析。结果:克隆了HSA-GHRH融合基因,构建了pPIC9-HSA-GHRH融合表达载体;电击转化后通过表型筛选和诱导表达实验得到蛋白表达工程菌;经分离纯化后,对表达产物的生物学活性分析显示其在体内有促进生长的作用。结论:与人血清白蛋白的融合有效地提高了GHRH的表达水平,并延长了GHRH的半衰期。     

Distribution of isotopic label after the oral administration of free and bound 14C-labelled glucosamine in rats

The metabolic fate of [1-(14)C]glucosamine, of N-acetyl[1-(14)C]glucosamine and of glycoproteins labelled with [1-(14)C]glucosamine was studied in rats for a period of 24hr. after these materials were given orally or injected. When [1-(14)C]glucosamine was injected 26.3% of the label was excreted in the urine, 19.7% was expired as carbon dioxide and 12.7% was incorporated into plasma proteins. When the same compound was given orally, 49.2% of the label was expired as carbon dioxide, with little appearing in the urine or in the plasma. When N-acetyl[1-(14)C]glucosamine was injected, 51.3% of the label was excreted in the urine with 12.3% appearing in carbon dioxide, but there was little incorporation into plasma protein. When this compound was given orally, 46.5% of the label was expired as carbon dioxide, 7.4% was recovered in the urine and 1.7% was incorporated into plasma protein. After the injection of (14)C-labelled glycoprotein 21.0% of the label was expired as carbon dioxide, whereas when it was given orally 49.8% of the label was recovered in carbon dioxide. The differences observed between the metabolic fate of the amino sugars when they were given orally and their fate when injected could not be accounted for by the action of the intestinal microflora or by the rate of administration of the material. It is concluded that amino sugars undergo metabolic alteration or degradation during absorption.     

秋水仙碱诱变甜菊多倍体的研究

用０．１％秋水仙碱溶液处理甜菊实生苗生长点,可诱变产生甜菊多倍体（四倍体）植株,用８次点滴处理,诱变率可达３１．２５％。染色体数鉴定表明：四倍体甜菊染色体数是２ｎ＝４４,而二倍体甜菊染色体数是２ｎ＝２２．形态学和解剖学的观察表明,四倍体比二倍体甜菊植株的茎矮壮,叶片增大,长度增长２．１倍,宽度扩大２．３倍,叶片加厚１．７倍,叶色更浓绿,叶片气孔数减少,气孔变大。叶片糖苷含量测定表明：四倍体的叶片含量为１５．７％,而二倍体的叶片含量为１０．８％,前者比二倍体叶片含量提高４．９％。     

青蛤的营养成分分析与评价

测定了61、2月份青蛤(Cyclina sinensis)的营养成份,并对其营养价值进行综合评定。结果表明,6月份青蛤的营养较12月份好,其粗蛋白比12月的高出2.84%,粗脂肪含量高出1.74%;6月和12月的氨基酸总含量分别为826.3 mg/g蛋白质和804.0 mg/g蛋白质,其中必需氨基酸分别占36.1%和33.6%,氨基酸计分(AAS)和化学评分(CS)是6月的较高,必需氨基酸指数(EAAI)则分别为64.23和59.88。其不饱和脂肪酸占脂质总量的67.7%,其中单烯酸占24.9%,多烯酸占42.8%,“脑黄金”DHA和EPA的含量分别达到11.3%和18.4%。还含有多种微量元素和维生素。     

粗柄独尾草不同器官蒽醌类成分的消长规律

采用高效液相色谱法对沙生类短命植物粗柄独尾草苗期、营养生长期、初花期、盛花期、果期各器官中大黄素、大黄酚、大黄酸、芦荟大黄素含量的消长规律进行了研究。结果表明:叶中,芦荟大黄素的含量在苗期和初花期都较高,在盛花期时最低;大黄酸的含量在苗期最高,盛花期时最低;大黄素的含量在苗期达到最高,初花期和盛花期最低;大黄酚的含量也以苗期最高,盛花期和果期最低。且在初花期时,4种蒽醌类物质含量均呈现明显的叶先端>叶中部>叶基部的空间差异性。根中,芦荟大黄素的含量在苗期和营养生长期较高,而以盛花期和果期较低;大黄酸的含量在果期最高,其余时期差异不显著;大黄素的含量以苗期和初花期较高;大黄酚的含量在果期达最高,而盛花期时最低。同时期的根叶蒽醌含量相比,叶中的芦荟大黄素要高于根,而根中大黄酚含量要高于叶。同时期各器官蒽醌总量相比:叶>根>花>花葶。故若选取粗柄独尾草作为蒽醌类药材利用,建议最佳采集方式为采集初花期的叶先端部分。     

乌鸡酶解技术研究

采用猪胰脏作为胰酶的主要来源,对乌鸡的酶解工艺进行了研究。实验结果表明：酶反应的最适温度为４５℃,胰酶混合物的合适用量为乌鸡鲜肉重量的５％,反应１８小时达反应平衡,反应浓度以１ｋｇ鲜乌鸡２０００ｍｌ水为宜,反应过程中维持ｐＨ７．３即可,酶解产物经测定：氨基酸及可溶性短肽总含量高达１６．６１％,其中必须氨基酸含量占氨基酸总含量的５３％。     

Transient state kinetic studies of phosphorylation by ATP and Pi of the calcium-dependent ATPase from sarcoplasmic reticulum.

The ATPase of the sarcoplasmic reticulum is phosphorylated by ATP in the presence of Ca2+. A rapid phosphorylation was observed when the enzyme was preincubated with Ca2+ prior to the addition of 0.1 or 1 mM ATP. The rate of phosphorylation was decreased when Ca2+ was omitted from the preincubation medium and added with ATP when the reaction was started. The rate of phosphorylation by ATP was further decreased when Pi was included in the preincubation medium without Ca2+. In this case, the enzyme was phosphorylated by Pi during the preincubation. When Ca2+ and ATP were added, a burst of phosphorylation by ATP was observed in the initial 16 ms. In the subsequent incubation intervals, the phosphorylation by ATP was synchronous with the hydrolysis of the phosphoenzyme formed by Pi. The rate of hydrolysis of the phosphoenzyme formed by Pi was measured when either the Pi concentration was decreased 10 fold, or when Ca2+, ATP or ATP plus Ca2+ was added to the medium. Upon the single addition of Ca2+, the time for half-maximal decay was in the range 500--1000 ms. In all other conditions it was in the range 70--90 ms.     

LRP16影响宫颈癌Siha细胞对化疗药物的敏感性

目的:探讨抑制LRP16的表达对宫颈癌Siha细胞的化疗药物敏感性的影响。方法:将抑制LRP16表达的小干扰RNA:negativecontrol-si RNA(NC)、si RNA-374(si374)转染入Siha宫颈鳞癌细胞系中,通过顺铂(DDP)和紫杉醇(TAX)的处理后,采用CCK-8检测不同浓度紫杉醇、顺铂作用宫颈癌细胞系Siha48 h后,计算出细胞被抑制一半时顺铂、紫杉醇的药物浓度(IC50);使用Hoechst33342染色观察细胞凋亡,采用流式细胞仪检测顺铂IC50作用Siha细胞48小时后的细胞凋亡情况,紫杉醇IC50作用Siha细胞之后的细胞周期分布情况。结果:CCK-8检测转染的Siha细胞增殖活性受到抑制,Hoechst33342染色观察转染的Siha细胞凋亡明显增加,流式细胞仪检测凋亡显示,si374+顺铂的早期凋亡率22.15±2.24,NC+顺铂12.45±2.72,流式细胞仪检测周期显示G2/M(%),si374+紫杉醇29.94±1.87,NC+紫杉醇17.66±2.32。结论:LRP16基因表达下调之后,抑制Siha细胞的增殖、促进其凋亡,使细胞周期滞留于G2/M期,从而提高Siha细胞的化疗敏感性。