979 resultados para AK-002-002
Resumo:
在野外模拟降雨条件下,比较研究了黄土丘陵区柠条(Caragana korshinkii)和狼牙刺(Sophora viciifolia)径流小区产流产沙、侵蚀泥沙颗粒组成、比表面积(SSA)及养分流失特征。结果表明,两种灌木群落均能显著减小坡面径流泥沙的流失。产流后流失泥沙黏粒、SSA与养分含量随降雨时间总体呈现降低趋势,其中有机质变化显著,全磷变化不显著。受植被盖度影响,泥沙中黏粒与养分含量均表现为柠条群落>狼牙刺群落>对照裸地。侵蚀泥沙具有富集黏粒和富集养分的特征,富集率随群落盖度增大而增大(柠条>狼牙刺>裸地)。不同形态养分富集率不同,其中有机质均在2.5以上,全氮平均富集率为2.13,全磷为1.23。富集率随产流时间呈线性递减。流失泥沙养分含量与黏粒(粒径<0.002 mm)含量及SSA达到极显著的正相关。坡面土壤养分主要以黏粒为载体流失。SSA的变化不仅能体现土壤颗粒组成的变化,而且能够反映土壤养分的变化。
Resumo:
毛细管电泳以其强大的分离能力日益受到重视,特别是成功完成人类基因组计划的测定工作,随着微全分析系统的深入研究,毛细管电泳的理论和技术在各方面都需要突破,其中毛细管电泳检测器是制约发展毛细管电泳更广泛地用于实际工作的因素之一。本论文以发展新型的毛细管电泳电化学发光检测技术为出发点,在以下几个方面作了研究。1.三联吡啶钌在玻碳电极上的阴极电化学发光我们首次发现了一种新型的基于溶液中氧的还原引发的三联毗淀钉(TBR)阴极电化学发光,结果表明,这种阴极电化学发光的发光电位仅为-0.4V,从而大大地降低了电化学发光的激发电位。所有能够增强阳极电化学发光的物质如三丙胺(TPA)都能够增强阴极电化学发光。阴极电化学发光光谱证实,阴极发光是激发态的TBR跃迁回到基态所产生的发光行为,我们认为在电极上氧还原所产生的活性氧氧化了TBR分子和发光增强剂从而导致了阴极发光。一些不能够增强阳极电化学发光的物质如柠檬酸,也能够增强阴极电化学发光,从而扩展了电化学发光的检测范围。采用阴极电化学方法对TPA和柠檬酸根的检测结果表明,对TPA在1*10~(-7)-1*10~(-5)M之间的检测呈较好线性相关性,相关系数为0.9994,最低检测限(S/N=3)为7.5*10-8M,对柠檬酸根在1*10~(-5)-1*10~(-4)M之间呈较好的线性关系,相关系数为0.999,最低检测限(S/N=3)为1.2*10~(-6)M。2.毛细管电泳直接电化学发光离柱检测技术的研究研究在没有场分离器的情况下高压电场对电化学发光检测器的影响。基于此目的我们采用75件m内径的毛细管为分离柱,300μm直径的铂丝为工作电极,以不同电导率的溶液作为电泳流动相。在高压电场的影响下,动态循环伏安和与此相对应的电化学发光表明电泳电流并不会引起电化学发光信号的淬灭,高压电场只会导致电化学发光激发电位向更正方向的偏移。进一步的研究表明,毛细管与工作电极之间的间距是影响电化学发光信号和理论塔板数的重要因素。基于以上的认识,我们发展了无需电场分离器的毛细管电泳一电化学发光检测系统,从而大大地简便了毛细管电泳一电化学发光检测系统。以三丙胺(TPA)作为分析对象,对该系统进行了表征,该系统对TPA的检测在1*10~(-10)-1*10~(-5)mol/L之间的线性相关系数为0.998,峰高的相对标准偏差为5.6%,检测限(S加=3)达到5.0*10~(-11)mol/L。采用这一方法对尿样中的利多卡因进行了分析,在5.0*10~(-8)-1.0*10~(-5) mo/L之间的相关系数为:0.998,最低检测限(S/N=3)为2.0*10-8mo/L。3.毛细管电泳一固态电化学发光检测器检测的研究我们首次报道将TBR固定在聚苯乙烯磺酸-溶胶-凝胶-接枝共聚物构成的膜中,采用旋涂的方法涂敷在铂电极的表面,制备用于毛细管电泳的固态电化学发光检测器,以TPA和脯氨酸作为研究对象表征了毛细管电泳-固态电化学发光检测系统的特征,该系统可以稳定工作24小时,完全可以满足实际应用的需要。采用该系统实现了对TPA和脯氨酸的同时检测,对TPA和脯氨酸检测的相对标准偏差分别为8.7%和7.5%,分离的理论塔板数分别为70000和16000,对TPA和脯氨酸的测定的最低检测限分别为0.002μM和2μM。4.离散小波分析去除毛细管电泳电化学发光检测信号的噪音毛细管电泳电化学发光检测信号因为TBR与溶液中的氢氧根的化学发光反应使得信号的噪音变得很大,从而影响了峰的定量,降低了检测灵敏度。这里我们采用离散小波'分析技术去除电泳中的噪音。对一些典型的小波基如HaaroDaublets,Coiflets和Symmlets去除噪音的效果作了比较。各种不同的计算阀值的方法和确定阀值的技术导致的去噪结果的差异作了比较。结果表明,采用Symmlet 4小波基和启发式无偏向风险估算法-软阀门确定阀值是最优的去噪方案,采用这一策略对毛细管电泳电化学发光电泳信号的去噪结果表明,噪音成功地得到了去除,同时电泳的峰型和轮廓得到了保留,该去噪技术明显地优于通常的SG和FT去噪技术。5.毛细管电泳柱端电化学发光同时检测尿样中的曲马多和利多卡因曲马多和利多卡因是手术中常用的镇静剂和麻醉剂,部分药物以原形从肾脏排除,我们研究了简单、快速的采用毛细管电泳柱端电化学发光同时检测曲马多和利多卡因的方法。我们使用25μm内径的毛细管作为分离柱,由于使用的毛细管内径很小,从而大大地降低了分离电压对检测器的影响,因此毛细管与电化学发光检侧器直接连接而无需电场分离器。使用300μm直径的铂盘电极作为工作电极,使得在毛细管的出口有足够的氧化态的TBR存在。为消除尿样中的离子强度对分析造成的影响,样品在分析前经萃取分离,以TPA为内标,采用两步萃取寻去对尿中的曲马多和利多卡因的测定回收率分别为94-96%和93-97%。在1.0*10-7to 1.0*10-4的浓度范围内曲马多和利多卡因的检测的线性相关系数为0.998,检测的相对标准偏差分别为2.9%和2.7%,对尿中曲马多和利多卡因测定的最低检测限(S/N=3)分别为6.0*10~(-8)mol/L和4.5*10~(-8)mol/L。应用该方法对临床两例术后病人尿样中的曲马多和利多卡因的代谢进行了测定。6.毛细管电泳电化学发光检测尿样中的利血平提出了一种快速、简便的毛细管电泳电化学发光法测定尿样中的利血平的方法。我们以25拼m内径的毛细管为分离柱,不用场分离器直接与300μm直径的铂二〔作电极连接,为提高检测的灵敏度和克服尿样中的离子强度对检测的影响,我于门采用场放大电动进样的技术用于毛细管电泳的直接进样和分离,样品不经任何预处理。由于利血平是中性分子,采用毛细管区带电泳不能将利血平与中性的干扰物分离出,因此我们在电泳流动相中加入十二烷基磺酸钠(SDS),成功地将利血平与中性干扰物质分离开。该方法对尿样中的利血平检测范围在l*10~(-6)~(-1)*10~(-4)mol/L 比的线性相关系数为0.996,相对标准偏差为4.3%,最低检测限为7.0*10~(-8)mol/L。
Resumo:
生物燃料电池作为一种真正意义上的理想绿色环保电源,由于可作为小功率长寿命的体内植入电源,已成为人们研究的热点课题之一。目前对生物燃料电池的研究主要集中在间接型生物燃料电池,已取得一定进展。但是间接型生物燃料电池具有电子传递链长、效率低等弱点,而直接型生物燃料电池有望克服以上缺点,成为更具研究潜力的新一代生物燃料电池。本文从探索简单、有效的酶固定方法入手,制备炭载辣根过氧化物酶(HRP)、漆酶(Lac)、酪氨酸酶(Tyr)作直接型生物燃料电池的阴极催化剂和炭载葡萄糖氧化酶(GoD)作阳极催化剂。用多种谱学方法表征了炭载酶催化剂的结构特征和用电化学方法研究了炭载酶的直接电化学及电催化性能。得到的主要结果和结论如下:1.以比活性高、稳定、结构清楚、有纯的商品化试剂且价廉的HRP为模型分子来探索用平衡吸附法将HRP固定到活性炭表面,用Nofion膜加固并修饰到玻碳(GC)电极上,以期制备得到炭载HRP修饰的Gc电极(HRP-C/GC)。实验结果表明,炭载HRP能进行准可逆的直接电化学反应,式电位(0)在50-700mv/s的范围内几乎不随扫速变化,平均值为C0.362±0.001)v,表观速率常数(ks)为(3.4±0.69)s-1HRP-C/GC电极对HZoZ还原有很好和稳定的电催化活性,表明固定在活性炭上的HRP能保持其生物活性,而且能稳定数月时间。因此,固定在活性炭上的HRP有可能用作直接型生物燃料电池的阴极催化剂。由上述结果可见,用平衡吸附法把HRP固载到活性炭上,并用Nofion膜加固的酶电极的制备方法具有简单且有效的特点,有可能作为直接型生物燃料电池酶催化剂的制备方法。2.用平衡吸附法将Lac和Tyr分别固定到活性炭上,发现炭载Lac和Tyr都能进行准可逆的直接电化学反应,其0,在10-150mv/s的范围内几乎不随扫速而变化,分别为-0.166和-0.139v。另外,还发现炭载Lac和Tyr对02的还原有明显的电催化作用,表明炭载Lac和Tyr仍能保持它们的生物活性,因而能作直接型生物燃料电池的阴极催化剂。3.用平衡吸附法将葡萄糖氧化酶(GOD)固定到活性炭表面,发现炭载GOD能进行准可逆的直接电化学反应,其0,在10-200mv/s的范围内几乎不随扫速而变化,平均值为C0.467±0.002)v;ks值为(1.18±0.59)5-1;且其直接电化学反应是2e+ZH+的过程。另外,还发现炭载GOD对p-D(+)葡萄糖的氧化有明显的电催化作用,表明炭载GOD没有发生变性,仍保持其生物活性,所以能用作直接型生物燃料电池的阳极催化剂。
Resumo:
氢化物发生-高频感耦等离子体原子发射光谱分析(HY-ICP-AES),由于它的灵敏度高和多元素同时分析等特点,近年来受到越来越多的科学工作者的重视。本文对HY-ICP-AES的原理、发展及应用作了比较详细的综述,并根据氢化物元素和非氢化物元素同时测定的实际要求,提出了一种新型的氢化物发生-雾化系统。文献上已报导了两种氢化物元素和非氢化物元素同时测定的方案,并取得了令人满意的结果。但在这些方案中,存在一些问题需要解决,而且装置比较复杂,操作也比较麻烦。在我们的氢化物发生-雾化系统中,用一个同心玻璃雾化器将待测的样品溶液雾化,细雾滴形成气溶胶,较大液滴被收集在一个玻璃槽中,硼氢化钾溶液用蠕动泵从玻璃槽底部送入,与收集的样品溶液混合并发生化学反应,产生挥发性的共价氢化物。生成的气态氢化物和样品气溶胶以及载气一起进入等离子体,因而可以进行氢化元素和非氢化物元素的同时测定。砷、锑、硒和碲的检出限分别为0.0075,0.0006,0.008,0.003,0.002 μg/ml,比传统的气动雾化方法得到的检出限好20-30倍。而对非氢化物元素,检出限可与双简雾室雾化相当。本系统进样量小(约2 ml),且样品的利用率大为提高,有利于小量样品的分析。但由于进样量较小,限制了灵敏度的进一步提高。本系统的另一个特点是不仅可以用于氢化物元素和非氢化物元素的同时测定,而且在需要的情况下,不需拆换雾化装置,不需灭火,即可在1-2分钟内转变成为普通的测定非氢化物元素的雾化系统。只要将蒸馏水取代硼氢化钾溶液把收集样品溶液的玻璃槽冲洗干净,即可作为普通的雾化系统之用。我们用这种氢化物发生-雾化系统研究了等离子体功率、载气流量、观测高度、样品介质酸度、硼氢化钾溶液和流量对待测元素信号强度、信-背比和检出限的影响以及硼氢化钾溶液的稳定性和硼氢化钾的引入量对等离子体稳定性的影响等。我们还研究了几种共存干扰元素对氢化物形成的干扰情况。为了消除或减小共存元素对氢化物生成过程的干扰,我们试验了EDTA,8-羟基喹啉,氨三乙酸,硫脲等对干扰元素的掩蔽作用,最后选EDTA作为掩蔽剂,对消除或减小共存元素的干扰起了明显的作用。我们用本雾化系统分析了一种甜菜颗粒粕样品和桃叶82301标准参考物质。分析结果与其它方法或标准值比较吻合。在甜菜颗粒粕样品的分析中,我们发现基体中大量镁、钙对砷等低含量元素的光谱干扰比较严重,利用元素间干扰比不能予以准确扣除。我们用标准和样品的基体相匹配的方法解决了镁、钙的光谱干扰问题。
Resumo:
The composition and microstructure of buried layers of AlN formed by high energy N+ ion implantation into polycrystalline Al have been determined. Both bulk and evaporated thin films of Al have been implanted with 100 and 200 keV N+ ions to doses of up to 1.8 x 10(18)/cm2. The layers have been characterised using SIMS, XTEM, X-ray diffraction, FTIR, RBS and in terms of their microhardness. It is found that, for doses greater than the critical dose, buried, polycrystalline AlN layers are formed with preferred (100) or (002) orientations, which are sample specific. With increasing dose the nitrogen concentration saturates at the value for stoichiometric AlN although the synthesised compound is found to be rich in oxygen.
Resumo:
采用脉冲激光沉积工艺在不同条件下以Si(111)为衬底制备了Zno薄膜.通过对不同氧压下(0~50Pa)沉积的样品的室温PL谱测试表明,氧气氛显著地提高了薄膜的发光质量,在50Pa氧气中沉积的ZnO薄膜具有最强的近带边UV发射.XRD测试说明在氧气氛中得到的薄膜结晶质量较差,没有单一的(002)取向.利用-低温(500℃)沉积的ZnO薄膜作缓冲层,得到了高质量的ZnO外延膜.与直接沉积的ZnO膜相比,生长在缓冲层上的ZnO膜展现出规则的斑点状衍射花样,而且拥有更强的UV发射和更窄的UV峰半高宽(98meV).对不同温度下沉积的缓冲层进行了RHEED表征,结果表明,在600~650℃之间生长缓冲层,有望进一步改善ZnO外延膜的质量.
Resumo:
采用双晶X射线衍射(DC-XRD)研究蓝宝石(0001)衬底上横向外延GaN层中晶面倾斜的形成原因。发现横向生长区的GaN在垂直掩模方向上朝SiNx掩模层弯曲。采用选择性腐蚀逐渐去掉SiNx掩模层,发现XRD中G N(002)ω扫描衍射峰两侧存在与晶面倾斜有关的衍射信息。该衍射信息起初为一个很宽的峰,随着选择性腐蚀的进行,会先分裂为两个峰,最后当SiNx掩模层全部腐蚀掉后,其中一个衍射峰会消失,而只剩下一个很窄的峰。作者证实造成横向外延GaN中晶面倾斜的原因有两个
Resumo:
尝试用侧向外延(ELOG)方法来降低立方相GaN中的层错密度。侧向外延是在SiO_2/GaN/GaAs图像形底上进行的,对生长所得的立方相GaN外延层用扫描电子显微镜(SEM)和透射电子显微镜(TEM)进行了观察和分析,TEM的平面像表明经过ELOG方法生长后,立方相GaN外延层中的层错密度由侧向外延生长前的5 * 10~9cm~(-2)降低至生长后的6 * 10~8cm~(-2)。双晶X射线衍射(DCXRD)测量给出侧向外延前后外延层ω扫描(002)衍射摇摆曲线的半高宽(FWHM)分别为33’和17.8’,表明晶体质量有了较大改善。对立方相GaN侧向外延过程中层错减少的机制进行了讨论。
Resumo:
High quality cubic GaN (c-GaN) is grown by metalorganic vapor deposition (MOCVD) at an increased growth temperature of 900 ℃, with the growth rate of 1.6 μm/h. The full width at half maximum (FWHM) of room temperature photoluminescence (PL) for the high temperature grown GaN film is 48meV. It is smaller than that of the sample grown at 830 ℃. In X-ray diffraction (XRD) measurement, the high temperature grown GaN shows a (002) peak at 20° with a FWHM of 21'. It can be concluded that, although c-GaN is of metastable phase, high growth temperature is still beneficial to the improvement in its crystal quality. The relationship between the growth rate and growth temperature is also discussed.
Resumo:
采用常规磁控溅射方法,通过优化工艺,在Si(100),Si(111)多种基片上沉积ZnO薄膜。利用透射电镜(TEM)、X射线衍射(XRD)和X射线摇摆曲线(XRC),对ZnO薄膜的微区形貌、结晶情况、C轴择优取向进行了详细的测试分析。结果表明,所制备的ZnO薄膜具有理想的结构特性,大多数样品测得ZnO(002)晶面XRC的半高宽(FWHM)1°左右,最小值达0.353°,优于目前国内外同类研究的最佳结果2°。并对ZnO/Si(100)与ZnO/Si(111)衬底的结果进行了比较和讨论。
Resumo:
以回摆法衍射峰的积分强度为基础,提出了X射线衍射分析单晶体时的多重性因子和衍射几何因子的概念,推导出普遍适用的相含量计算公式。利用双晶X射线多功能四圆衍射仪测绘GaN/GaAs(001)外延层中立方相(002)面、{111}面和六角相{10-10}面的极图和倒易空间Mapping,分析了六角相和立方相微孪晶的各晶面在极图中的分布特征及计算相含量时的多重性因子和衍射几何因子,并根据立方相(002)、立方相微孪晶{111}、六角相{10-11}和{10-10}衍射峰的积分强度,求得外延层中立方相微孪晶和六角相的含量。
Resumo:
Cubic GaN(c-GaN) films are grown on GaAs(001) substrates by metalorganic chemical vapor deposition (MOCVD). Two GaN samples were grown with different buffer layer, the deposition time of each was 1 and 3 min, respectively. 4-circle X-ray double crystal diffraction (XRDCD) was used to study the secondary crystallographic phases presented in the c-GaN films. The phase composition of the epilayers was determined by X-ray reciprocal space mapping. The intensities of the c-GaN(002) and h-GaN(10 (1) over bar 1) planes detected in the mapping were investigated by omega scans. The content of the hexagonal phase inclusions in the c-GaN films was calculated to about 1.6 and 7.9%, respectively. The thicker buffer layer is not preferable for growing high quality pure c-GaN films. (C) 2000 Elsevier Science S.A. All rights reserved.
Resumo:
为了从分子水平对中国药用石斛及其混伪品进行鉴定,本文选取了核rDNA ITS 序列和叶绿体DNA 的matK 基因序列进行研究。采用改良的CTAB 法提取石斛的基因组DNA,PCR 产物直接测序法对17 种(共32 份)药用石斛的核糖体内转录间隔区ITS 全序列进行测定,克隆测序法对12 种(共22 份)药用石斛的叶绿体的matK 基因序列进行测定,运用BioEd it,MEGA4.0 等生物软件分析了石斛属植物的rDNA ITS 序列及叶绿体的matK 基因序列的特征,比较了石斛属间、种间、种内不同居群(品种)间的序列碱基差异及遗传距离,应用邻接法构建分子系统树。主要研究结果如下: (1)建立了17 种(共32 份)药用石斛rDNA ITS 区碱基全序列数据库,其中,ITS1 的长度为228~234 bp,GC 含量为45.7%~53.0%,变异位点167 个,占总位点67.34%,信息位点106 个,占总位点42.74%,ITS2 长度为241~247 bp,GC含量为44.8%~55.7%,变异位点165 个,占总位点66.27%,信息位点115 个,占总位点46.18%。 (2)建立了12 种(共22 份)药用石斛的叶绿体matK 基因全序列数据库,叶绿体matK 基因长1410 bp,变异位点51 个,信息位点11 个。除了存在碱基替换的遗传变异外,还存在碱基的插入和缺失。 (3)通过ITS 序列比较分析了各材料间的遗传距离和碱基差异,属间的遗传距离为0.295,石斛种间的平均遗传距离为0.142,碱基相差2~156 个,种内各居群间的平均遗传距离为0.002,碱基相差1~2 个。属间的遗传距离大于种间的遗传距离,种间的遗传距离大于种内不同居群(品种)间的遗传距离。 (4)根据分析石斛叶绿体的matK 基因序列得到,外类群(密花石豆兰)与石斛属间最小遗传距离为0.027,石斛种间的平均遗传距离为0.008,种间最大的遗传距离0.014, 最小的遗传距离为0.003,碱基相差8~20 个。种内不同居群(品种)遗传距离为0.001,相差1~5 个碱基。 (5)利用17 种石斛的全序列数据库及遗传分析软件,通过对待检种rDNA I TS区进行序列测定,成功地对10 个待检种进行了鉴定,并且在原植物开花后得到了验证。 (6)运用12 种石斛的matK 基因全序列数据库及遗传分析软件,成功地对4个待检种进行了鉴定,同样在原植物开花后得到了验证。 (7)本文利用石斛的核糖体内转录间隔区ITS 序列和叶绿体的matK 基因序列数据库分别构建了NJ 树,外类群与石斛属间石斛种间以及种内不同居群(品种)间均能在NJ 树中明显分化开来,二者构建的分子系统树一致,为石斛的分子鉴定提供了依据。 In order to identify Chinese Herba Dendrobii and its adulterant species on molecular level, we studied the sequences of rDNA ITS and chloroplast matK gene. Genomic DNA of Dendrobium was extracted using the modified cetyltrimethyl ammonium bromide (CTAB) method. The PCR products of the rDNA ITS sequences of Dendrobium (32 materia ls) were purified and then sequenced. The PCR products of chloroplast matK gene of Dendrobium (22 materia ls) were purified, cloned and then sequenced. The characteristic of the sequences and the genetic dista nce were compared between Bulbophyllum odoratissimum and Dendrobium, Dendrobium interspecies, and different populations. Phylogenetic trees were constructed using the NJ method by the biology softwares including BioEd it, MEGA4.0 etc. The ma in results as follows: (1) It was built up that the database of rDNA ITS sequences of 17 species of Herba Dendrobii (32 materia ls). The ITS1 was 228~234 bp, the GC content accounting for 45.7%~53.0%. Its variable sites were 167, accounting for 67.34%. The Parsim-Informative positions were 106, accounting for 42.74%. The ITS2 was 241~247 bp, the GC accounting for 44.8%~55.7%. The variable sites were 165, accounting for 66.27%. The Parsim-Informative positions were 115, accounting for 46.18%. (2) The database of the chloroplast matK gene sequences was built up, which contained 12 species of Herba Dendrobii (22 materia ls). The matK gene sequences were about 1410bp in length. There were 51 variable sites and 11 Parsim-Informative sites. And there were nucleotides insertions and deletions in some species , in addition to the nucleotides substitutions. (3) The rDNA ITS sequences were compared and analyzed by the biology softwares. The genetic dista nce between Bulbophyllum odoratissimum and Dendrobium was 0.295. The avera ge genetic dista nce was 0.142 between Dendrobium species, and there were 2~156 variable nucleotides. The avera ge genetic dista nce between different populations was 0.002, and there were 2~156 variable nucleotides. The genetic dista nce between Bulbophyllum odoratissimum and Dendrobium was greater tha n that of Denrobium interspecies. Meanwhile, the genetic dista nce between Denrobium species was also greater tha n that of different populations (variaties). (4) The characteristics of the chloroplast matK gene sequences were obtained after analyzing by the biology softwares. The minima l genetic dista nce was 0.027 between Bulbophyllum odoratissimum and Dendrobium . The ma xima l genetic dista nce was 0.014 between Dendrobium species, and there were 20 variable nucleotides. The minima l genetic dista nce between populations was 0.003, and there were 8 variable nucleotides.The genetic dista nce between populations was 0.001, and there were 1~5 variable nucleotides. (5) The molecular Phylogeny tree was constructed on the database of rDNA ITS the sequences of 17 species of Herba Dendrobii using the biology softwares. Then we authenticated 10 materia ls on molecular level. What’s more, they had been proved when these pla nts flowered. (6) The molecular Phylogeny tree was built up on the database of chloroplast matK gene sequences of 12 species of Herba Dendrobii with the biology softwares.Then 4 materia ls were authenticated on molecular level. Moreover, they had also been proved when these pla nts were in flower. (7) The Phylogenetic trees were separately constructed on the sequences of rDNA ITS and chloroplast matK gene B. odoratissimum and Dendrobium all could be distinguished on the Phylogenetic trees. Meanwhile, the Phylogenetic trees based on two groups of sequences were coincident. rDNA ITS and matK gene sequence could be used as molecular markers for authentication of Herba Dendrobii.
Resumo:
本文从不同厌氧生境中获得7组(C-2、Y-2、L-2 、NZ、H-3、CZ、L-3)具有纤维素降解能力的复合菌系。经过不断传代、淘汰纤维素降解能力降低的菌系,最后得到一组高效、传代稳定的厌氧纤维素分解复合菌系L-3。该菌系可使滤纸在42 h内溃烂,并能在分解纤维素的同时产氢气。对L-3复合菌系的产酶条件进行了研究,结果表明,在实验范围内该菌系的产酶最适条件为:pH 6.5,温度37 ℃,接种量5 %,最佳碳源为滤纸,最佳氮源为硫酸铵。第10天测得羧甲基纤维素酶(CMCase)、滤纸酶(FPA)、外切葡聚糖酶(C1)、β-葡聚糖苷酶(β-glucodase)的酶活分别为0.216 U/ml、0.101 U/ml、0.132 U/ml、0.002 U/ml,滤纸失重率70.6 %。发酵代谢产物乙醇和丁酸含量分别可达1378 mg/L 、2695 mg/L,发酵产生的气体中氢气含量最高可达70.2 %。DGGE结果表明该菌系主要由14种菌组成,其中有三株菌在发酵前后菌数发生了明显的变化,说明在以滤纸为底物的降解过程中,这三株菌起到了重要作用,对这三株菌进行了分子生物学鉴定,初步定为Clostridium phytofermentans、Clostridium cellulovorans、Desulfovibrio sp。 利用实验室分离得到的纤维素降解菌,最终配制出由10、X-1、X-13、ST-13、L-3组成的好氧-厌氧纤维素降解复合菌剂。以秸秆为发酵底物,菌剂接种量1%,利用复合菌剂预处理后的秸秆,发酵总产气量相对于对照提高了71.62%,甲烷含量最高可达70.08%。 A group of microbial consortia L-3 was isolated from the anaerobic fermentation residue of corn stalk, which could degrade cellulose and produce hydrogen. The CMCase, FPA, C1 and β-glucosidase activity of L-3 could reach to 0.216 U/ml, 0.101 U/ml, 0.132 U/ml and 0.002 U/ml, respectively. In the filter degrading process, the filter paper collapsed in the liquid culture within 42 h and the filter degrading rate could reach to 70.6% in the 13 days, meanwhile, hydrogen was determined and the highest hydrogen content was 70.2%. The optimum cellulase-degrading conditions were filter papaer as the carbon source, (NH4)2SO4 as the nitrogen source, 37 ℃ and pH 6.5 in this experiment. DGGE results showed that the microbial consortia L-3 mainly included 14 strains. The amount of 3 strains were changed during the fermentation. These strains were identified as Clostridium phytofermentans、Clostridium cellulovorans、Desulfovibrio sp by 16S rDNA sequence analysis. The cellulose- degrading microbial agent was composed by 10, X-1, X-13, ST-13, L-3 which were isolated in the laboratory. The straw pretreated by cellulose-degrading microbial agent was used to ferment, the total biogas production increased by 72% comparing to the control. The content of methane could reach to 70.08%。
Resumo:
本论文研究了利用三孢布拉氏霉(Blakeslea trispora)发酵产β-胡萝卜素的培养条件。主要包括:发酵培养基的确定,发酵条件的优化。还考察了发酵菌丝体中β-胡萝卜素的提取方法及薄层层析等。 首先研究了培养基成分对三孢布拉氏霉发酵产β-胡萝卜素的影响。确立了玉米淀粉作为碳源,黄豆粉(热榨)作为氮源,棉籽油作为植物油的发酵培养基配方,其成分为:玉米淀粉 3%,黄豆粉(热榨) 2%,棉籽油 3%,KH2PO4 0.2%,MgSO4·7H2O 0.2%,维生素B1 0.002%,pH值6.0。 其次,通过比较不同的发酵影响因子,分别得到最适的条件:如三孢布拉氏霉正负菌接种比例为1.3:0.7,培养基pH值为7.0(灭菌后),发酵促进因子为Triton X-100。并采用正交试验法,确定其最佳发酵条件为正负菌接种比例1.3/0.7,发酵培养基pH为7.0,在培养基中添加表面活性基Triton X-100 0.08%。使该菌株产β-胡萝卜素的量达到0.73g/L,较初始发酵条件提高了3.3倍。 研究中还找到一个简便有效的对β-胡萝卜素的提取方法,选用盐酸-热处理法进行细胞破壁,并选用沸程为60~90℃的石油醚进行萃取。 用三孢布拉霉菌丝体内类胡萝卜索的石油醚提取液点样于硅胶G板,以丙酮:石油醚(5:95)为展开剂能将β-胡萝卜素与其它类胡萝卜索分离。该方法简便快速,并有一定实用价值。 The fermentative conditions of β-carotene by Blakeslea trispora have been investigated. These conditions include fermentation medium, the optimization of some fermentation factor. The extracting methods and the TLC of carotenoids were also researched. Firstly, the effects of composition of fermentation medium on the yield of β-carotene were studied. the results showed that the best fermentation medium was corn starch 3%,soybean power 2%,cottonseed oil 3%,KH2PO4 0.2%,MgSO4·7H2O 0.2%,vitamin B1 0.002%,pH value 6.0. Secondly, through compared some factors, such as different proportion of plus and minus strains, pH value, nonionic surfactants, respective best values have been obtained. The best proportion of plus and minus strains is 1.3:0.7, pH value of fermentation medium (sterilized) is 7.0, fermentation accelerant which acts as surfactants is Triton x-100. Farther on, the fermentative conditions were optimized through orthogonal experiment, the optimization showed that proportion of plus and minus strains is 1.3:0.7,pH value is 7.0, content of Triton x-100 is 0.08%. And the yield of β-carotene reached 0.73g/L, which was up to 3.3 times through the fermentation. In the extracting study, it has showed hydrochloric acid-heat treatment is a simple, convenient and effective extracting methods is which was used to destroy the cell wall, and the extracting organic solvent is petroleum ether whose boiling range is 60~90 ℃. In the TLC experiments, extracting contents in the petroleum ether were spotted in the silicagel plate, and the mixed liquor of acetone and petroleum ether (5:95) is developping agent, which can distinguish β-carotene from other carotenoids. It is a simple and quick technique.
