转基因红花中角质细胞生长因子KGF-1的表达

通过构建重组表达质粒载体p139035S-KGF1和根癌农杆菌介导在红花(Carthamus tinctorius)中表达角质细胞生长因子(KGF-1)。从侵染到诱导生根共需要14周, 转化率达0.1%。红花子叶在潮霉素筛选培养基上培养4–5周后便可获得丛生芽, 再生芽移入含潮霉素的伸长生根培养基, 培养4–8周可诱导生根。通过PCR、Southern blot、RT-PCR及Western blot检测证明目的基因KGF-1已经整合到红花细胞的染色体中, 实现了KGF-1外源蛋白在红花中的成功表达, 为开发KGF-1蛋白新的生产途径奠定了基础。     

番茄ACC合酶反义基因对河套蜜瓜的转化

河套蜜瓜（CucumismeloLcvHetau）的子叶经预培养。芽诱导和生根培养,获得再生小植株,诱导率达58％。取带有番茄ACC合酶反义基因的双元载体pMQ6／JM109与农杆菌（Agrobacteriumtumefaciens）LBA4404经三亲融合后,与在MS0上萌发5d、并在MS＋1mg／LNAA培养基上预培养3d的子叶共培养48h,然后转入含50mg／L卡那霉素的MS＋6mg／LZT的芽诱导培养基中,1l个月后诱导生芽,待芽长1．5－2cm时转入生根培养基中,1－2周后可诱导产生大量的根,形成完整的转基因小植株。经PCR和分子杂交检测证明,目的基因已整合入河套蜜瓜的基因组中。     

红花荷的组织培养与快速繁殖

1植物名称红花荷（Rhodoleia championii Hook.f.）,别名红苞木、吊钟王。2材料类别茎段。3培养条件以MS为基本培养基。（1）芽诱导培养基：MS＋6-BA2.0mg·L^-1（单位下同）＋IBA0.5;（2）丛生芽诱导及增殖培养基：MS＋6-BA0.5＋IAA0.2＋AC（活性炭）0.5;（3）生根培养基：1/2MS＋6-BA0.5＋IAA0．2＋AC0．5。以上培养基中均加入3％的蔗糖、     

重组HIV-1壳体蛋白在转基因枸杞根系中的分泌表达

P24壳体蛋白（capsid, CA）是HIV¬-1早期感染的一个重要标志.用含有植物表达载体pCAMBIA 1305.2- MA4-CA（包含GRP信号肽和MA4-CA融合基因）的农杆菌菌株侵染枸杞,将转有MA4-CA融合基因的转化株诱导生根，并进行毛状根的培养; western blot证实根系及培养液中的MA4-CA融合蛋白以二聚体的形式存在，分子量为50 kDa；免疫组织化学显示，CA定位在细胞浆、细胞壁和细胞间隙中，充分证实了利用GRP信号肽可以引导重组蛋白分泌表达。建立枸杞中HIV-1壳体蛋白的根分泌表达系统，为研究植物HIV-1 CA-病毒样颗粒（VLPs）疫苗奠定基础。     

提高成年云南山楂树试管培养苗生根率的方法

用成年云南山楂(Crataegus scabrifolia(Franch)Rehd.树的无菌增殖芽苗作为生根试验材料。结果表明：接种在含生长素(IBA、NAA)0.01-1.0mg/1的MS/2培养基中,芽苗的平均生根率为50.4%;在高浓度(150-250mg/1)生长素溶液中浸泡芽苗基部30分钟,然后接种到无生长素的MS/2培养基中,其生根率为60.1%;用高浓度生长素液蘸芽苗基部的生根率为83.5%;芽苗在含IBA1-5mg/1的培养基中培养2-4天,然后转入MS/2培养基中诱导生根,生根率可达92%以上,根伸长正常。黑暗条件明显抑制生根,每日16小时至24小时光照对芽苗生根有益。     

铁核桃离体培养与快速繁殖

以优良单株‘纳雍-1’的单芽茎段为外植体,建立了铁核桃（Juglanssigillata）离体培养与快速繁殖的体系。结果表明,附加6-BA1．0mg·L-1 ＋活·IgK（AC）3．0g·L-1的DKw培养基适宜铁核桃腋芽诱导;适宜铁核桃芽增殖的培养基为DKW＋6-BA1．0mg·L-1 ＋IBA0．02mg·L-1,40d后增殖系数可达7．33;试管苗的茎尖和茎段均可用于增殖培养;一步生根法（低浓度的生长素IBA持续诱导）不利于铁核桃试管苗嫩茎生根;采用二步生根法,生根率最高可达71．73％,其中,不同IBA浓度、暗培养时间、蔗糖浓度和AC含量对试管苗嫩茎生根影响显著,铁核桃试管苗在附]sulBA5,0mg·L-1的1／4DKW培养基中暗培养12d,再转移到不含IBA的1／4DKW培养基（附加AC 3g-L-1和蔗糖20g·L-1）中生根效果最好;生根试管苗采用珍珠岩和营养土两步炼苗,60d后成活率达到87．50％。     

PEG法介导转化诸葛菜下胚轴原生质体获得转基因植株

采用诸葛菜无菌苗的下胚轴组织为材料,分离原生质体,在原生质体培养基中作液体浅层暗培养,植板率为５％,植株再生频率为１００％。作者进而开展了遗传转化研究。为研究ＰＥＧ介导转化诸葛菜原生质体的影响因素,通过瞬间表达,实验了ＰＥＧ法转化子叶原生质体的过程,在此基础上将分离纯化后的原生质体与带ＨＰＴ基因的质粒ＤＮＡ（ｐＢＩ２２２）混合,ＨＰＴ基因作选择标记,ＰＥＧ介导转化;重新收集转化后的原生质体,以５×１０４／ｍｌ的密度在原生质体培养基中作浅层培养;培养１０—１５天后用２５ｍｇ／Ｌ的潮霉素（ｈｙｇｒｏｍｙｃｉｎ）进行筛选,一月后出现少量细胞团,转入含潮霉素５０ｍｇ／Ｌ的扩增培养基扩增愈伤组织,进而转入含５０—１００ｍｇ／Ｌ潮霉素的分化培养基诱导分化成苗,分化率为１００％,转入生根培养基中生根成完整植株。抗性植株再生率为４×１０（－５）。在获得再生转基因植株后,以再生植株叶片为材料,进行Ｓｏｕｔｈｅｒｎｂｌｏｔ分子杂交,证实外源基因已稳定整合到植物基因组中并表达,再生转基因植株频率为１０（－５）。国内外首次转化诸葛菜属植物原生质体获得成功。     

盐地碱蓬幼嫩花序的组织培养及植株再生

选用盐地碱蓬(Suaeda salsa)幼嫩花序为外植体, 建立了快速而高效的离体培养体系。在附加1.0mg.L-16-BA和0.4 mg.L-1 IAA的MS培养基上培养25天可诱导出不定芽, 诱导频率达到82.1%; 不定芽在此培养基上可快速扩增和长期继代培养。不定芽转至MS培养基中培养2~3周生根形成完整植株。     

盐地碱蓬幼嫩花序的组织培养及植株再生

选用盐地碱蓬(Suaedasalsa)幼嫩花序为外植体,建立了快速而高效的离体培养体系。在附加1.0mg.L-16-BA和0.4mg.L-1IAA的MS培养基上培养25天可诱导出不定芽,诱导频率达到82.1%;不定芽在此培养基上可快速扩增和长期继代培养。不定芽转至MS培养基中培养2￣3周生根形成完整植株。     

红厚壳茎段丛生芽诱导与植株再生

红厚壳(Calophyllum inophyllum)为藤黄科红厚壳属多年生木本植物,有很高的药用价值。该研究以红厚壳带节茎段为外植体,探讨生长调节剂对腋芽萌发及丛生芽诱导、伸长和试管苗生根的影响。研究结果表明,外植体腋芽萌发和丛生芽诱导效果最好的培养基是MS+NAA1.0+TDZ0.5,在此条件下培养21天后,转入添加0.5 g·L–1活性炭且无生长调节剂的MS培养基,可有效促进不定芽的伸长。将带不定芽的外植体先在附加1.0 mg·L–1NAA的1/2MS培养基上进行生根诱导4周,之后转入附加1.0 g·L–1活性炭的无激素培养基进行根的伸长培养,这样的两步生根法能有效促进红厚壳生根。     

Mass production of pure gibberellin A1 by Phaeosphaeria sp. L487 and the fungal preparation of [U-13C]gibberellin A1.

The mass production of pure gibberellin A1 (GA1) by shake-culturing Phaeosphaeria sp. L487 was investigated. Its GA1 production was markedly influenced by natural nitrogen sources and NH4NO3. When the fungus was cultured in an 8% glucose-1.5% oatmeal-0.1% NH4NO3-0.5% KH2PO4-0.1% MgSO4 x 7H2O medium for 3 weeks, the amount of GA1 in the culture filtrate was up to ca. 200 microg/ml: the addition of safflower oil to the culture medium two weeks after inoculation prolonged the GA1-production period to produce 300 microg/ml. Further preparation of [U-13C]GA, as a tool for the analysis of a complex of GA1 and its binding protein was attempted by using the fungus. The fungal culture in a [U-13C]glucose-oatmeal medium gave 6 mg of crystalline 13C-enriched GA1. Its 13C-enrichment of ca. 75% and 1J(CC) values were determined by NMR spectrometry.     

An increase in liver PPARγ2 is an initial event to induce fatty liver in response to a diet high in butter: PPARγ2 knockdown improves fatty liver induced by high-saturated fat

The effects of a diet rich in saturated fat on fatty liver formation and the related mechanisms that induce fatty liver were examined. C57BL/6J mice were fed butter or safflower oil as a high-fat (HF) diet (40% fat calories) for 2, 4, 10, or 17 weeks. Although both HF diets induced similar levels of obesity, HF butter-fed mice showed a two to threefold increase in liver triacylglycerol (TG) concentration compared to HF safflower oil-fed mice at 4 or 10 weeks without hyperinsulinemia. At 4 weeks, increases in peroxisome proliferator-activated receptor γ2 (PPARγ2), CD36, and adipose differentiation-related protein (ADRP) mRNAs were observed in HF butter-fed mice; at 10 weeks, an increase in sterol regulatory element-binding protein-1c (SREBP-1c) was observed; at 17 weeks, these increases were attenuated. At 4 weeks, a single injection of adenoviral vector-based short hairpin interfering RNA against PPARγ2 in HF butter-fed mice reduced PPARγ protein and mRNA of its target genes (CD36 and ADRP) by 43%, 43%, and 39%, respectively, with a reduction in liver TG concentration by 38% in 5 days. PPARγ2 knockdown also reduced mRNAs in lipogenic genes (fatty-acid-synthase, stearoyl-CoA desaturase 1, acetyl-CoA carboxylase 1) without alteration of SREBP-1c mRNA. PPARγ2 knockdown reduced mRNAs in genes related to inflammation (CD68, interleukin-1β, tumor necrosis factor-α, and monocyte chemoattractant protein-1). In conclusion, saturated fatty acid-rich oil induced fatty liver in mice, and this was triggered initially by an increase in PPARγ2 protein in the liver, which led to increased expression of lipogenic genes. Inactivation of PPARγ2 may improve fatty liver induced by HF saturated fat.     

激肽释放酶转基因大鼠模型的建立

目的建立KLK1转基因大鼠模型。方法腹腔注射PMSG-HCG（150-150IU/kg）超排不同周龄（4-8周）SD大鼠比较超排效果的差异,以可用于注射胚胎数作为评判标准确定最佳超排周龄。构建pBC-klk1转基因构件,经酶切、纯化后通过显微注射方法导入SD大鼠受精卵原核并移植到同期受孕的SD受体母鼠输卵管内。出生后仔鼠用PCR和Southern方法检测鼠尾DNA鉴定基因型,通过RT-PCR和免疫组化方法检测klk1基因表达。结果4-8周SD大鼠超排后分别获得受精卵14±14.8、30±15.2、13.3±13.7、13±14.7、8±5.7,5周龄大鼠超排效果最好,与其他周龄大鼠相比有显差异,P〈0.05;显微注射1538枚卵,移植685（44.53%）枚卵于31只受体输卵管中,12（12/31,38.7%）只怀孕,共产仔62只,经PCR检测获得6只阳性鼠,Southern检测3只阳性。对Southern检测阳性转基因大鼠子代进行RT-PCR检测和免疫组化分析证明klk1基因在肾脏、胰腺和乳腺内表达。结论成功建立klk1基因表达的转基因大鼠模型,该模型是高血压病研究的理想动物模型。     

Dietary fat modulation of apoA-II metabolism and prevention of senile amyloidosis in the senescence- accelerated mouse

Senescence-accelerated mouse-prone (SAMP1; SAMP1@Umz) is an animal model of senile amyloidosis with apolipoprotein A-II (apoA-II) amyloid fibril (AApoAII) deposits. This study was undertaken to investigate the effects of dietary fats on AApoAII deposits in SAMP1 mice when purified diets containing 4% fat as butter, safflower oil, or fish oil were fed to male mice for 26 weeks. The serum HDL cholesterol was significantly lower (P < 0.01) in mice on the diet containing fish oil (7.4 +/- 3.0 mg/dl) than in mice on the butter diet (38.7 +/- 12.5 mg/dl), which in turn had significantly lower (P < 0.01) HDL levels than mice on the safflower oil diet (51.9 +/- 5.6 mg/dl). ApoA-II was also significantly lower (P < 0.01) in mice on the fish oil diet (7.6 +/- 2.7 mg/dl) than on the butter (26.9 +/- 7.3 mg/dl) or safflower oil (21.6 +/- 3.7 mg/dl) diets. The mice fed fish oil had a significantly greater ratio (P < 0.01) of apoA-I to apoA-II, and a smaller HDL particle size than those fed butter and safflower oil. Severe AApoAII deposits in the spleen, heart, skin, liver, and stomach were shown in the fish oil group compared with those in the butter and safflower oil groups (fish oil > butter > safflower oil group, P < 0.05). These findings suggest that dietary fats differ in their effects on serum lipoprotein metabolism, and that dietary lipids may modulate amyloid deposition in SAMP1 mice.     

尿酸性肾病中IL-1beta、IRAK-4 的表达及意义

目的：通过研究尿酸性肾病动物模型中白介素-1(IL-1)beta和白介素-1受体相关激酶4(IRAK-4) 表达的意义,了解IL-1beta信号 通路在尿酸性肾病中的作用。方法：Wistar 大鼠54 只随机分为高尿酸血症组30 只、正常组24 只,制备尿酸性肾病大鼠模型,检测 尿酸(UA)、尿素氮(BUN)、肌酐(CR)及肌酐清除率(Ccr)、24 h尿微量白蛋白(mA1b);取肾脏组织行HE 染色,观察形态学变化;免疫 组化测定IL-1beta的表达;荧光定量PCR 检测IRAK-4 mRNA的水平。结果：高尿酸组2、4、6 周时IL-1beta的表达均增加,免疫组化评 分(IHS)均明显升高(P<0.01);高尿酸血症组较正常组IRAK-4 mRNA 在2、4、6 周时均出现表达上调,4～6 周IRAK-4 mRNA表达 明显增加,与正常组比较有显著性差异(P<0.01)。结论：IL-1beta、IRAK-4 参与了尿酸性肾病炎症反应的过程,可能为尿酸性肾病治疗 提供新的可能。     

注射用红花黄色素辅助治疗早期糖尿病肾病的临床效果观察

目的：观察注射用红花黄色素辅助治疗早期糖尿病肾病（diabetic nephropathy,DN）的临床效果。方法：选择2011年10月至2012年2月我院收治的早期DN患者86例,在患者知情同意的情况下随机分为对照组（n=42例）和观察组（n=44例）,对照组采取西医常规治疗措施,观察组在上述治疗措施的基础上加用注射用红花黄色素治疗,治疗4周后,比较两组患者的实验室检查指标及临床疗效。结果：治疗4周后,观察组患者的白蛋白排泄率（UAER）、尿β2微球蛋白（β2-MG）、血肌酐（Scr）、血尿素氮（BUN）、血甘油三酯（TG）、血胆固醇（TC）、低密度脂蛋白（LDL）均显著低于对照组,差异均具有统计学意义（P〈0.05）;对照组治疗总有效率为85.7%,观察组治疗总有效率为97.7%,两组患者治疗总有效率比较,差异具有统计学意义（P〈0.05）,观察组优于对照组。结论：注射用红花黄色素治疗辅助治疗早期DN可有效其提高临床疗效。     

链脲佐菌素诱导C57小鼠1型糖尿病模型的研究

目的:通过小剂量多次腹腔注射链脲佐菌素(STZ)诱导建立与人类1型糖尿病相似的C57小鼠糖尿病模型,研究建模剂量和成模率。方法:将32只C57小鼠随机分为正常对照组(A)和实验组(B)。实验组(B)可分为低、中、高剂量组(50 mg/kg、70mg/kg、90 mg/kg)(n=8)。两组都喂普通饲料1周后,B组连续5天腹腔注射不同剂量STZ,测定注射前、注射后1周、2周、3周、4周、5周的空腹血糖和体重,观察小鼠饮食、饮水和排尿情况。STZ注射第3周进行口服糖耐量实验(OGTT)。结果:给药前A、B组体重和血糖无显著差异,给药1周后,B组饮水量和进食量明显增加,体重减轻。C57小鼠用药2周后,中剂量组达到建模标准,成模率75%。各剂量组均出现了糖耐量异常。结论:诱导建立C57小鼠1型糖尿病模型方法是连续5日腹腔注注射STZ,适宜剂量为70 mg/kg。