883 resultados para Recycled PET


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以蛋白质为基础的分析生物器件,如传感器和生物芯片等,为人们提供了有效的分析技术平台。而蛋白质固定的均质性则是评估分析生物器件质量的一个主要指标。因此,本实验以两种蛋白质为模式蛋白研究蛋白质固定的均质性问题。通过基因操纵构建融合蛋白Protein-Linker-Cysteine。在此设计中,半胱氨酸提供的自由疏基能够在金表面形成Au一S键,在琉基修饰的玻片表面形成-S-S-键实现蛋白质的均质定向固定;Linker可减少基因修饰对蛋白质折叠的影响。构建表达载体pPIC-GOxm(GOx-Linker-Cysteine),利用原生质体转化法将其转进毕氏酵母Pichia Pastoris,采用QSepharoseTM FastFlow阴离子交换柱纯化融合蛋白。动力学性质分析表明GOxm具有与野生型葡萄糖氧化酶相类似的Km和Kcat值,电化学实验结果显示Goxm传感器具有较高的响应电流;GOxm传感器具有较好的互换性,其相对误差为9.48%,GOxw(wild type GOx)相对误差为19.98%,而传统传感器的相对误差为17.54%。原子力显微镜图像显示融合蛋白GOxm能够利用金表面的HC尸位点形成类似六边型晶格的自组装单分子层,而野生型GOxw在金表面为非特异性吸附,形成多层固定导致分子间的聚集。通过利用-S-S-和非特异性吸附,分别制成GOxm蛋白芯片和Goxw蛋白芯片。酶学显色后,通过光学信号评估芯片的均质性,结果表明Goxm能够利用-S-S-形成均质定向固定,10次重复的变异系数小于60k,而GOxw则不能形成均质固定,点阵间的变异系数变化幅度非常大,从40%到80%。构建表达载体pET-BLC,pET-BL。将其转化进大肠杆菌AD494中。原子力显微镜研究整合有磷脂和经抽提去掉磷脂的蛋白在金表面的固定。原子力显微镜图像显示融合蛋白BLC能够利用Au-S键在金表面形成均匀固定,而野生型蛋白在金表面不能形成均匀的固定。蛋白质在金表面的固定受金表面拓扑结构和磷脂的影响。以上的实验结果表明通过此种固定方法可改善分析生物器件的均质性,提高其质量。

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以PCR技术从金黄色葡萄球菌基因组DNA中首次克隆编码成熟SECZ蛋白的全基因sec2。该基因共717bp,编码239个氨基酸,Genbank Accession number:AY450554。构建了SEC2的表达载体pET-28a-sec2,并在大肠杆菌BL21(DE3)中高效表达可溶性rSEC2蛋白。经亲和层析纯化,其纯度在95%以上,平均回收量为每升培养物40mg。纯化的rSEcZ保持了与野生型相当的生物学活性。以限制性核酸内切酶连接技术分别将两个抗人表皮生长因子受体HER-2单链抗体基因通过DNA Linker与sec2融合,构建融合基因b-l-sec2和ml小sec2,并以两种方式表达纯化。以pET-32a表达载体在E,coliAD494(DE3)中以氨基端融合大肠杆菌硫氧还蛋白(TrxA)形式高效表达融合蛋白TRX-B-L-SEC2和TRX-ML-L-SEC2,经亲和层析纯化,并以肠激酶切割得到成熟融合免疫毒素B-L-SEC2和ML-L-SEC2,其纯度在95%以上,平均回收量为每升培养物smg;以构建的新型表达载体pASK-75-EX在E.coliBL21(ED3)中以不溶性包涵体形式表达融合免疫毒素蛋白,经变性、纯化和复性后得到具有生物学活性的融合免疫毒素,其纯度在95%以上,平均回收量为每升培养物30mg。以两种方式制备的融合免疫毒素都保持了SECZ蛋白的免疫原性,都能有效刺激人外周血单个核细胞的增殖,并且都显示出在体外与HER-2过表达的乳腺癌细胞SK-Br-3特异性结合能力,具有显著的靶向性抑瘤作用。用PcR方法扩增了编码TrxA蛋白的基因trxA并克隆至表达载体pET-28a启动子上游,构建了一种在单质粒中利用两个相同的启动子游离共表达硫氧还蛋白与目的蛋白的表达载体。利用该载体可使TrxA与外源蛋白在大肠杆菌BL21(DE3)中以非融合形式高效共表达。共表达的TrxA可明显促进外源蛋白单链抗体ML3.9(scFv-ML)、3一轻基苯甲酸-6-单加氧酶(3HBA)的可溶性表达;并明显减少肠毒素C2(SEC2)、结核杆菌螺旋酶A亚基(GYRA)的包涵体表达。

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本文以青藏高原东部的高山草甸为研究对象,设置早融、中间及晚融三个融雪部位,采用实验室测量、野外测量、野外样方调查相结合的 方法,从个体、种群和群落的水平上比较研究了高山雪场植物在同一雪场样地中不同融雪梯度上的特征变异及适应,结果表明: 从早融到晚融的梯度上,随着融雪时间的逐渐推迟,表土日温差降低,冻融交替的强度减弱,土壤水份逐渐增加,总N、总P、总K 以及 可溶性的N、P 和pH 变化不明显,土壤有机质及可溶性的K 和Ca 逐渐降低。冻融交替强度上的差异以及土壤水分差异被认为是融雪梯度上 影响植物生长的主要原因。 从早融到晚融的梯度上,伴随着生态因子的改变,几种常见植物的个体特征也发生相应的变化。首先,物候期推迟。植物开始生长的时间 一般要推迟将近二十天,但同一种植物在不同的融雪部位上的衰老期趋于一致,这预示着在晚融部位同一植物的生长期要缩短。其次,个体生 长特性发生改变。黑褐穗苔草(Carex atrofusca subsp. minor (Boott) T.Koyama)和西北黄芪(Astragalus fenzelianus Pet.-Stib.)的个体生长(株高、单株叶数、单叶面积和地上生物量)表现为逐渐增加的趋势;斑唇马先蒿(Pedicularis longiflora Rudolph var. tubiformis (Klotz.) Tsoong)和川西小黄菊(Pyrethrum tatsienense (Bur. et Franch.) Ling ex Shih.)则表现为逐渐降低的趋势;长叶火绒草(Leontopodium longifolium Ling)在融雪梯度上的变化趋势不明显。再次,从繁殖特性来看,大卫马先蒿(Pedicularis davidii var. pentodon Tsoong)的单株花数、单花种子数、种子千粒重及种子萌发率随融雪的推迟呈现为逐渐增加的趋势;圆穗蓼(Polygonum macrophyllum D.Don)的种子(小坚果)千粒重和萌发率也表现为逐渐增加,其余繁殖特征变化不明显。 在种群层次上,几个常见物种的分布格局随着融雪的推迟都发生一定的变化,基本上表现为从早融的集群分布到中间或晚融部位的随机分布。物种间的联结性也发生较大的变化,由早融部位的总体上的正关联逐步过度到晚融部位上的总体上的负关联。特定种对间的联结性也发生较大的变化。恶劣环境条件(如剧烈的冻融交替)的影响以及对恶劣条件适应被认为是分布格局及种间联结性发生变化的主要原因。 在群落层次上,物种多样性的变化表现为单峰曲线的格局,即在中间部位多样性最高。早融部位强烈的冻融交替和晚融部位缩短的生长季是早融及晚融部位物种多样性不高的重要原因。几乎所有的只出现在一个融雪部位(雪深级别)上的物种都发生在中间融雪部位。这说明,中等的雪深更有利于许多高山植物的存活,而过浅过深的积雪都不利于植物的生存。另外,相距较近的融雪梯度之间的物种相似性较大,而相距较远的梯度之间物种的替代率较高,物种的相似性较小。在群落的生物量方面,地上生物量随融雪的推迟而升高,地下生物量随融雪的推迟而下降,地上与地下生物量之总和随着融雪的推迟而下降,地下生物量与地上生物量之比随着融雪的推迟而下降。早融部位的地上生物量主要集中于地上0-10cm 的范围内,表明在早融部位植物地上部分有变矮的趋势;早融部位的地下生物量在土壤各深度分布相对较均一,而晚融部位地下生物量则主要集中于地下0-10cm 的范围内。生物量的变化趋势主要与雪场中各部位的土壤水分含量及地表日温度差异有关,是植物适应特定环境的结果。 To detect the plants’ responses to snow-cover gradients in an alpine meadow of eastern Tibetan plateau, laboratory method and field sample plot method were employed, and three gradeients (early-, medium and late-melting)were established in a natural snowbed. The measurements were carried out for two years and was done on three levels——individual, population and community. The results are shown as follows : From early- to late-melting gradients, daily ground temperature difference between day and night decreased, amplitude of freeze-thaw alternation weakened, soil organic matter contents and soluble K and Ca decreased, while soil water content increased. Total N, total P, total K,pH soluble N and soluble P kept constant from early- to late-melting portions. Among these factors, the changes of intense freeze-thaw alternation and soil water contents were considered as main factors affecting plants’ growth. From early- to late-melting portions, all phenological phases postponed, e.g. phase of plant emergence postponed almost twenty days. However, the same species’ individuals at different portions withered in step, which implied that the individuals at late-melting portion possessed shorter growing season length. Along the same gradient, both Carex atrofusca subsp. minor (Boott) T. Koyama and Astragalus fenzelianus Pet.-Stib. increased their individual growth, whereas Pedicularis longiflora Rudolph var. tubiformis (Klotz.) Tsoong and Pyrethrum tatsienense (Bur. et Franch.) Ling ex Shih. decreased their individual growth. Unlike the four plants mentioned above, Leontopodium longifolium L. did not show any evident change. As to reproductive charateristics, the flowers per individual, the number of seeds per flower, the thousand seed weight and the seed germination rate of Pedicularis davidii var. pentodon showed an increasing trend; and Polygonum macrophyllum D.Don also increased its thousand seed weight and seed germination rate along the same gradient. However, the other reproductive charateristics of Polygonum macrophyllum D.Don did not change significantly. At population level, the distribution pattern of several selected species changed from cluster pattern to random pattern as the snowmelt postponed. Overall association among the species changed from positive to negative along the same gradient. Further, interspecific association also changed evidently. Adverse circumstances such as intense freeze-thaw alternation were considered as primary factors resulting in changes of population distribution pattern and interspecific association. At the level of community, species diversity showed a pattern of a unimodal trend, i.e. the highest diversity occurred at medium snow depth,perhaps because of intense freeze-thaw alternation at early-melting portions and the shortest growing season at late-melting portions. Almost all species that only appeared at one snowmelt portion occurred at medium portion, indicating that medium snow depth was more suitable for many species’ survival. Species replacement from one snowmelt portion to its neighboring portion seldom took place. However, while distance between two portions became farther, species replacement between the two portions occurred more frequently. As for biomass, aboveground biomass increased from early- to late-melting portions, whereas belowground biomass, total biomass and the ratio of belowground to aboveground all decreased along the same snow gradient. A majority of aboveground biomass distributed in a height range of 0-10 cm, suggesting that height of plants inhabiting early-melting portion be shorter compared with other portions. In addition, belowground biomass at early-melting portion was evenly distributed at different soil depth in comparison with aboveground biomass, whereas belowground biomass at late-melting portion concentrated 0-10cm soil layer below ground. The changing trend of biomass was also related to two factors. One was soil water content, and the other topsoil temperature difference between day and night.

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高等植物种子胚乳贮藏蛋白是种子发芽时的主要氮源,也是人类和动物食用植物蛋白的主要来源。大麦种子胚乳贮藏蛋白主要是醇溶蛋白(hordeins),占大麦胚乳总蛋白的50–60%。根据大麦醇溶蛋白的大小和组成特点,大麦醇溶蛋白被划分为三种类型:富硫蛋白亚类(B,γ-hordeins)、贫硫蛋白亚类(C-hordeins)以及高分子量蛋白亚类(D-hordeins)。B组和C组醇溶蛋白是大麦胚乳的两类主要贮藏蛋白,它们分别占大麦总醇溶蛋白成分的70–80%和10–12%。遗传分析表明,大麦B、C、D和γ-组醇溶蛋白分别是由位于大麦第五染色体1H(5)上的Hor2、Hor1、Hor3和Hor5位点编码。Hor2位点编码大量分子量相同但组成不同的B组醇溶蛋白(B-hordein)。B-hordein的种类、数量和分布是影响大麦酿造、食用及饲养品质的重要因素之一。为深入了解B-hordein基因家族的结构和染色体组织,探明Hor2位点基因表达的发育调控机制,最终达到改良禾谷类作物籽粒品质的目的,本研究以青藏高原青稞为材料,采用同源克隆法,分别克隆B-hordein基因和启动子,通过原核生物表达验证B-hordein基因功能,并利用实时定量PCR探索B-hordein基因表达时空关系,取得如下研究结果: 1. 以具有特殊B组醇溶蛋白亚基组成的9份青藏高原青稞为材料,根据GenBank中三个B-hordein基因序列(GenBank No. X03103, X53690和X53691)设计一对引物,通过PCR扩增,获得23个B-hordein基因克隆并对其进行了序列分析。核苷酸序列分析表明,所有克隆均包含完整的开放阅读框。有11个克隆都存在一个框内终止密码子,推测这11个克隆可能是假基因。推测的氨基酸序列分析表明,所有大麦B-hordein具有相似的蛋白质基本结构,均包括一个高度保守的信号肽、中间重复区以及C-端结构域。不同大麦种重复区内重复基元的数目有较大差异。青稞材料Z07–2和Z26的B-hordeins仅具有12个重复基元结构,更接近于野生大麦。这些重复基元数目的差异导致了重复区序列长度和结构的变异。这种现象极可能是由于醇溶谷蛋白基因在进化过程中染色体的不平衡交换或复制滑动所造成的。对所克隆基因和禾本科代表性醇溶谷蛋白基因进行聚类分析,结果表明所有来自栽培大麦的B-hordeins聚类成一个亚家族,来自野生大麦的B-hordeins以及普通小麦的LMW-GS聚类成另外一个亚家族,表明这两个亚家族的成员存在显著差异。此外,我们发现B-hordein基因推测的C-末端序列具有一些有规律的特征:即具有相同C-末端序列的B-hordein基因在系统发生树中聚类为同一个亚组(除BXQ053,BZ09-1,BZ26-5分别单独聚为一类外)。这个特征将有助于我们对所有B组醇溶蛋白基因家族成员进行分类,避免了在SDS-PAGE电泳图谱上仅依靠大小分类的局限性。 2. 根据上述克隆的青稞B-hordein基因的5’端序列设计三条基因特异的反向引物,以青稞Z09和Z26的基因组DNA为模板,采用SON-PCR和TAIL-PCR技术分离克隆出8个B-hordein基因的上游调控序列(命名为Z09P和Z26P)。序列分析表明,推测的TATA box位于–80 bp,CAAT–like box位于–140 bp处。此外,Z09P和Z26P中有六个序列在–300 bp处均存在一个由高度保守的EM基序和类GCN4基序构成的胚乳盒(Endosperm Box,EB),在约–560 bp处存在一个胚乳盒类似结构。而Z09P-2和Z26P-3不存在保守的胚乳盒或其类似结构,预示着这两个启动子所调控的基因表达可能受不同类型反式作用因子的调节,推测该启动子对基因的表达调控具有多样性。 3. 将B-hordein基因的开放阅读框定向克隆到表达载体pET-30a中,将其导入大肠杆菌表达菌株BL21中进行外源基因的诱导表达以验证所克隆基因的功能。结果表明仅含重组子pET-BZ07-2和pET-BZ26-5的BL21细菌有目的表达蛋白产生。在诱导3 h时的蛋白表达量最高;3 mM IPTG诱导的蛋白表达量要高于1 mM IPTG诱导的表达量。这为分离纯化B-hordein蛋白以及进一步研究其对大麦籽粒品质的影响奠定基础。 4. 根据从青稞Z09和Z26中分离克隆的B-hordein基因序列设计一对基因特异的引物,同时,选择大麦α-微管蛋白基因(GenBank no. U40042)为看家基因并设计特异引物,利用实时荧光定量PCR检测了青稞籽粒4个胚乳发育时间段的B-hordein基因表达,荧光定量结果显示:两份材料中B-hordein基因的表达量均随发育过程的进行而逐渐升高。Z09中B-hordein基因在开花后7天开始转录,而Z26开花4天后就有低水平B-hordein的表达,这表明Z26中B-hordein基因可能比Z09表达的较早或者Z09中B-hordein基因表达水平较低以致于不能被检测到。此外,在4个不同的胚乳发育时期中,Z26中B-hordein基因的表达量均高于Z09材料。在开花12天到18天的过程中,Z09和Z26中B-hordein基因的表达水平有一个急剧性的升高。这说明在不同胚乳发育时期,Hor2位点的B-hordein等位基因变异体存在mRNA的差异表达。 Seed endosperm storage proteins in higher plants are the main resources of nitrogen for germinating and plant proteins for human and animals. Barley prolamins (also called hordeins) are the major storage proteins in the endosperm and account for 50–60% of total proteins. Hordeins are classically divided into three groups: sulphur-rich (B, γ-hordeins), sulphur-poor (C-hordeins) and high molecular weight (HMW, D-hordeins) hordeins based on the size and composition. B-hordeins and C-hordeins are two major groups and each respectively account for about 70-80% and 10-12% of the total hordein fraction in barley endosperm. Genetic analysis showed that B-, C-, C-, γ-hordeins are encoded by Hor2, Hor1, Hor3 and Hor5 locus on the chromosome 1H (5). Hor2 locus is rich in alleles that encode numerous heterogeneous B-hordein polypeptides. It is reported that B-hordein species, quantity and distribution are significant factors affecting malting, food and feed quality of barley. To understand comprehensively the structure and organization of B-hordein gene family in hull-less barley and explore the developmental control mechanisms of Hor2 locus gene expression and eventually to better exploitation in crop grain quality improvement, we isolated and cloned B-hordein genes and promotors of hull-less barley from Qinghai-Tibet Plateau by PCR, and testified their expression founction in bacteria expression system and explore their spatial and temporal expression pattern by quantitative real time PCR. Our results are as followed, 1. Twenty-three copies of B-hordein gene were cloned from nine hull-less barley cultivars of Qinghai-Tibet Plateau with special B-hordein subunits and molecularly characterized by PCR, based on three B-hordein genes published previously (GenBank No. X03103, X53690 and X53691). DNA sequences analyses confirmed that the six clones all contained a full-length coding region of the barley B-hordein genes. Eleven clones all contain an in-frame stop codon and they are probably pseudogenes. The analysis of deduced amino acid sequences of the genes shows that they have similar structures including signal peptide domain, central repetitive domain, and C-terminal domain. The number of the repeats was largerly variable and resulted in polypeptides in different sizes or structures among the genes. Twelve such repeated motifs were found in Z07–2 and Z26, and they are close to those of the wild barleys, and it is most probably caused by unequal crossing-over and/or slippage during replication as suggested for the evolution of other prolamins. The relatedness of prolamin genes of barley and wheat was assessed in the phylogenetic tree based on their polypeptides comparison. Our phylogenetic analysis suggested that the predicted B-hordeins of cultivated barley formed a subfamily, while the B-hordeins of wild barleys and the two most similar sequences of LMW-GS of T. aestivum formed another subfamily. This result indicated that the members of the two subfamilys have a distinctive difference. In addition, we found the B-hordeins with identical C-terminal end sequences were clustered into a same subgroup (except BXQ053,BZ09-1 and BZ26-5 as a sole group, respectively), so we believe that B-hordein gene subfamilies possibly can be classified on the basis of the conserved C-terminal end sequences of predicted polypeptide and without the limit of SDS-PAGE protein banding patterns. 2. The specific primers were designed according to the published sequences of barley B-hordein genes from Z09 and Z26. Using total DNA isolated from them as the templates, eight clones (designated Z09Pand Z26P) of upstream sequences of the known B-hordein genes was obtained by TAIL-PCR and SON-PCR. Sequences analysis shows that the putative TATA box was present at position –80 bp and CAAT-like box at position –140 bp. Besides, a putative Endosperm Box including an Endosperm Motif (EM) and a GCN4-Like Motif was found at position –300 bp in six clones, and another Endosperm-like box was found at positon –560 bp. While the Endosperm Box or Endosperm-like box was not found in Z09P-2 and Z26P-3. This may indicate that gene expression drived by the two promtors was probably controlled by different trans-acting factors and the genetic control mechanism of corresponding gene expression may be diverse. 3. The B-hordein genic region coding for the mature peptide was cloned into expression vector pET-30a and transformed into bacterial strain BL21 for identifying gene expression fountion. Protein SDS–PAGE analysis showed that only the transformed lysate with the pET-BZ07-2 and pET-BZ26-5 constructs produced proteins related to B-group hordeins of barley, and the mounts of proteins induced by 3 mM IPTG and 3 h were higher than other conditions. This established a base for isolating and putifying B-hordein and further exploring their effects on barley grain quality. 4. The gene-specific primers of B-hordein genes from Z09 and Z26 were used for the quantification of B-hordein gene expression. The α-tubulin gene from Hordeum vulgare subsp. vulgare (GenBank accession number U40042) was used as a control gene. The result shows the transcription of the B-hordein genes in Z09 was found 7 days after flowering, while the transcription of the B-hordein genes in Z26 was found 4 days after flowering, but at a very low level, and it suggested that the B-hordein genes in Z26 probably expressed earlier than those in Z09, or the B-hordein genes in Z09 expressed at so a lower level than Z26 that it can not detected. In addition, B-hordein genes in Z26 accession showed higher expression levels than those in Z09 in four developing stages. Furthermore, a progressive increase in the expression levels of the B-hordein genes between 12 and 18 days after anthesis was observed in both Z09 and Z26. It implies that the B-hordein allelic variants encoded by Hor2 locus exist the differential expression in mRNA levels of during barley endosperm development.

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株高是农作物的重要农艺性状之一,适度矮化有利于农作物的耐肥、抗倒、高产等。20世纪50年代,以日本的赤小麦为矮源的半矮秆小麦的培育和推广,使得世界粮食产量显著增长,被誉为“绿色革命”。迄今为止,已报到的麦类矮秆、半矮秆基因已达70多个,但由于某些矮源极度矮化或者矮化的同时伴随不利的农艺性状,使得真正运用于育种实践的矮源较少。因此,发掘和鉴定新的控制麦类作物株高的基因,开展株高基因定位、克隆及作用机理等方面的研究,对实现麦类作物株高的定向改良,具有重要的理论意义和应用价值。簇毛麦(Dasypyrum villosum,2n=14,VV)是禾本科簇毛麦属一年生二倍体异花授粉植物,为栽培小麦的近缘属。本课题组在不同来源的簇毛麦杂交后代中发现了一株自然突变产生的矮秆突变体。观察分析了该突变体的生物学特性,对矮秆性状进行了遗传分析,对茎节细胞长度、花粉的活力进行了细胞学观察,考察了该突变体内源赤霉素含量及不同浓度外施赤霉素对突变体的作用,分析了赤霉素生物合成途径中的内根贝壳杉烯氧化酶(KO)和赤霉素20氧化酶(GA20ox)的转录水平,对赤霉素20氧化酶和赤霉素3-β羟化酶(GA3ox)进行了克隆和序列分析,并对GA20ox进行了原核表达和表达的组织特异性研究。主要研究结果如下:1. 该突变体与对照植株在苗期无差异,在拔节后期才表现出植株矮小,相对对照植株,节间伸长明显受到抑制,叶鞘长度基本不变。在成熟期,对照植株的平均株高为110cm,而突变株的平均株高为32cm,仅为对照植株的1/3 左右。除了株高变矮以外,在成熟后期,突变株还表现一定程度的早衰和雄性不育。I2-KI染色法观察花粉活力结果表明,对照植株花粉90%以上都是有活力的,而突变植株的花粉仅20%左右有活力。2. 突变株与对照植株的杂交F1代均表现正常株高,表明该突变性状为隐性突变。F1代植株相互授粉得到的168株F2代植株中,株高出现分离,正常株高(株高高于80cm)与矮秆植株(株高矮于40cm)的株数比为130:38,经卡方检验,其分离比符合3:1的分离比,因此推测该突变体属于单基因的隐性突变。3. 用ELISA方法检测突变株和对照植株的幼嫩种子中内源性生物活性赤霉素(GA1+3)含量,结果表明突变株的赤霉素含量为36 ng/ml,而对照植株的赤霉素含量为900 ng/ml。对突变株外施赤霉素,发现矮秆突变株的株高和花粉育性均可得到恢复。这些结果表明该突变株为赤霉素缺陷型突变。4. 用荧光定量PCR方法比较突变株与对照植株中内根贝壳杉烯氧化酶和赤霉素20氧化酶的转录水平,结果表明突变株的KO转录水平比对照植株分别提高了6倍(苗期)和16倍(成熟期),突变株的GA20ox转录水平与对照植株在苗期无明显差异,在成熟期突变株较对照植株则提高了10倍左右。这些结果表明该矮秆突变体与赤霉素的生物合成途径密切相关,而且极有可能在赤霉素的生物合成途径早期就发生了改变。5. 以簇毛麦总基因组为模板,同源克隆了GenBank登录号为EU142950,RT-PCR分离克隆了簇毛麦的GA3ox基因cDNA全长序列,分析结果表明该cDNA全长1206bp,含完整编码区1104bp,推测该序列编码蛋白含368个氨基酸残基,分子量为40.063KD,等电点为6.27。预测的氨基酸序列含有双加氧酶的活性结构,在酶活性中心2个Fe离子结合的氨基酸残基非常保守。该序列与小麦、大麦和水稻的GA3ox基因一致性分别为98%、96%、86%。基因组序列与cDNA序列在外显子部分一致,在478-715bp和879-1019bp处分别含238bp和140bp的内含子。6. 通过RT-PCR技术克隆了簇毛麦的GA20ox基因全长,命名为DvGA20ox,GenBank登录号为EU142949。该基因全长1080个碱基,编码359个氨基酸,具有典型的植物GA20ox基因结构。该基因编码的蛋白质与小麦、大麦、黑麦草等GA20ox蛋白的同源性分别为98%,97% 和91%。该序列重组到原核表达载体pET-32a(+)上,将获得的重组子pET-32a(+)-DvGA20ox转化大肠杆菌BL21pLysS后用IPTG进行诱导表达。SDS-PAGE分析表明,DvGA20ox基因在大肠杆菌中获得了高效表达,融合蛋白分子量为55kDa。定量PCR分析表明,该基因在簇毛麦不同器官中的表达差异明显:叶片中表达水平最高,根部表达水平次之,茎部和穗中表达较弱。在外施赤霉素后,该基因的表达水平在两小时以后急剧下降,表明该基因的表达受自身的反馈调节。本研究结果认为,(1)该簇毛麦矮秆突变体为单基因的隐性突变;(2)该矮秆突变体为赤霉素敏感突变,内源赤霉素含量检测表明突变体的内源性赤霉素含量仅为对照植株的1/30;(3)荧光定量PCR结果表明突变株的赤霉素生物合成途径的关键酶基因表达水平比对照植株高,而且突变植株的赤霉素生物合成改变很可能发生在赤霉素生物合成途径的早期;(4)GA20ox有表达的组织特异性,且受到自身产物的反馈调节。 Plant height is an impotrant agronomic trait of triticeae crops.Semi-dwarf cropcultivars, including those of wheat, maize and rice, have significantly increased grainproduction that has been known as “green revolution”. The new dwarf varieties couldraise the harvest Index at the expense of straw biomass, and, at the sametime, improvelodging resistance and responsiveness to nitrogen fertilizer. Moreover, dwarf traits ofplant are crucial for elucidating mechanisms for plant growth and development aswell. In many plant species, various dwarf mutants have been isolated and theirmodles of inheritance and physiology also have been widely investigated.The causesfor their dwarf phenotypes were found to be associated with plant hormones,especially, gibberellins GAs.Dasypyrum villosum Candargy (syn.Haynaldia villosa) is a cross-pollinating,diploid (2n = 2x = 14) annual species that belongs to the tribe Triticeae. It is native toSouthern Europe and West Asia, especially the Caucasuses, and grows underconditions unfavorable to most cultivated crops. The genome of D. villosum,designated V by Sears, is considered an important donor of genes to wheat for improving powdery mildew resistance, take-all, eyespot, and plant and seed storageprotein content. A spontaneous dwarf mutant was found in D. villosum populations.The biological character and modles of inheritance of this dwarf mutant are studied.The cell length of stem cell is observed. The influence of extraneous gibberellin tothe dwarf mutant is also examined; the transcript level of key enzyme of gibberellinbiosynthesis pathway in mutant and control plants is compared. GA3ox and GA20oxare cloned and its expression pattern is researched.1. The dwarf mutant showed no difference with control plants at seedlingstage.At mature stage, the average height of control plants were 110cm and the dwarfplants were 33cm. The height of the mutant plant was only one third of the normalplants due to the shortened internodes. Cytology observation showed that theelongation of stem epidermal and the parenchyma cells were reduced. The dwarfmutant also shows partly male sterile. Pollen viability test indicates that more than80% of the pollen of the mutant is not viable.2. The inheritance modle of this dwarf mutant is studied. All The F1 plantsshowed normal phenotype indicating that the dwarfism is controlled by recessivealleles. Among the 168 F2 plants, there are 130 normal plants and 30 dwarf plants, thesegregation proportion accord with Mendel’s 3:1 segregation. We therefore proposethat this dwarf phenotype is controlled by a single recessive gene.3. Quantitative analyses of endogenous GA1+3 in the young seeds indicated thatthe content of GA1+3 was 36ng/ml in mutant plants and 900ng/ml in normal plants.The endogenous bioactive GA1+3 in mutant plants are only about 1/30 of that innormal plants. In addition, exogenously supplied GA3 could considerably restore themutant plant to normal phenotype. These results showed that this mutant wasdefective in the GA biosynthesis.4. More than ten enzymes are involved in GA biosynthesis. KO catalyzes thefirst cytochrome P450-mediated step in the gibberellin biosynthetic pathway and themutant of KO lead to a gibberellin-responsive dwarf mutant. GA20ox catalyze therate-limited steps so that their transcript level will influence the endogenous GAbiosynthesis and modifies plant architecture. The relative expression levels of genesencoding KO and GA20ox were quantified by real time PCR to assess whether thechanges in GA content correlated with the expression of GA metabolism genes andwhere the mutant occurred during the GA biosynthesis pathway. In mutant plants,the transcript levels of KO increased about 6-fold and 16-fold at the seedling stage and elongating stage respectively comparing with the normal plants. For theseedlings, there was no notable difference in the expression of GA20ox betweenmutant and normal plants. At the elongating stage, GA20ox transcript increased 10times in mutant plants, suggesting that the GA biosynthesis pathway in mutant plantshad changed from the early steps rather than the late steps.5. A full length cDNA of D. villosum gibberellin 3β-hydroxylase homology(designated as DvGA3ox) was isolated and consisted of 1206bp containing an openreading frame of 1104bp encoding 368 predicted amino acid residues. Identityanalysis showed that the gibberellin 3β-hydroxylase nucleotide sequence shared 98%,96% and 86% homology with that of wheat, barley and rice. The predicted peptidecontained the active-site Fe of known gibberellin 3β-hydroxylase and the regionhomologous to wheat, barley and Arabidopsis. The genomic clone of gibberellin3β-hydroxylase has two introns.6. The full-length cDNA of D. villosum gibberellin 20 oxidase (designated asDvGA20ox) was isolated and consisted of 1080-bp and encoded 359 amino acidresidues with a calculated mol wt of 42.46 KD. Comparative and bio-informaticsanalyses revealed that DvGA20ox had close similarity with GA20ox from otherspecies and contained a conserved LPWKET and NYYPXCQKP regions. Tissueexpression pattern analysis revealed DvGA20ox expressed in all the tissues that wereexamined and the highest expression of DvGA20ox in expanding leaves followed byroots. Heterologous expression of this cDNA clone in Escherichia coli gave a fusionprotein that about 55KD. Transcript levels of DvGA20ox dramatically reduced twohours after application of biologically active GA3, suggesting that the biosynthesis ofthis enzymes might be under feedback control.

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首先简要回顾了重离子束治癌在我国的兴起与发展的情况。随后着重介绍了重离子束治癌装置及部分关键技术:总体布局方案、束流引出模式、束流配送系统、束流旋转机架、辐照门控系统、PET成像等。

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在室温和真空环境下利用不同的快重离子(1.158GeV Fe56、1.755GeV Xe136及2.636GeV U238)对多层堆叠的聚对苯二甲酸乙二醇酯(PET)、聚碳酸脂(PC)和聚酰亚胺(PI)进行了辐照,结合X射线衍射(XRD)、傅立叶红外光谱(FTIR)及紫外可见光谱测量技术,在较宽的电子能损(1.9-19.0 keV·nm-1)和注量范围(1×1010-6×1012 cm-2)研究了离子在不同聚合物潜径迹中引起的损伤过程,观测到了主要官能团的降解、炔基生成、非晶化及紫外吸收边缘的红移等现象随辐照注量及电子能损的变化趋势。通过对损伤过程的定量分析,应用径迹饱和模型假设,分别给出了Fe、Xe和U离子在不同电子能损下辐照PC时的平均非晶化径迹半径和炔基形成半径,并用热峰模型对实验结果进行了检验。

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重离子束治癌是重离子束在医疗领域中的一项典型的应用技术 .文章从重离子束在物理学与生物学上的特点 ,描述了它对肿瘤治疗具有的优越性 :物理剂量深度分布在射程末端有一个能量沉积集中区 ,其深度和大小均可调节 ;在靶区的相对生物效率 (RBE)高、氧增比 (OER)低 ;射程歧离与横向散射小 ;利用正电子发射断层照相 (PET)技术可以实时在线监测 ;可以三维扫描进行适形治疗 ;半致死损伤修复小 ;辐射敏感性不依赖细胞周期时相 .文章还介绍了这项技术的国内外进展 ,并对其未来进行了展望 .

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采用多种手段研究了 35Me V/u的 Ar离子辐照聚酯 (PET)膜产生的微观结构变化 .结果表明 ,辐照使聚酯的化学键断裂并产生了炔端不饱和基团和自由基 .断键主要发生在乙二醇残留物、苯环的对位和酯的 C— O键上 .随着吸收剂量的增加 ,材料的结晶度逐渐降低 ,由原始的41 .7%减至最高辐照量时的 1 5.0 % .研究发现 ,聚脂的非晶化转变截面与电子能损呈线性关系 ;断键和非晶化效应主要取决于样品的吸收剂量 ,并存在一个约 4.0 MGy的阈值

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用圆柱型流气式组织等效正比计数器测定了K 2 0 0kV低能重离子加速器提供的低能16O+离子束流在穿过 4μm厚的PET(C10 H8O4 )薄膜后的微剂量谱和径向剂量分布。测定了穿过不同厚度PET薄膜后的16O+ 束流的单次事件剂量平均比能zID随束流强度的变化曲线。用TIRM 92MonteCarlo程序计算了16O+ 离子在PET材料中的射程 ,与实验结果进行了比较和讨论

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This paper reports that the transmission of O6+ ions with energy of 150keV through capillaries in an uncoated Al2O3 membrane was measured, and agreements with previously reported results in general angular distribution of the transmitted ions and the transmission fractions as a function of the tilt angle well fitted to Gaussian-like functions were observed. Due to using an uncoated capillary membrane, our c is larger than that using a gold-coated one with a smaller value of E-p/q, which suggests a larger equilibrium charge Q(infinity) in our experiment. The observed special width variation with time and a larger width than that using a smaller E-p/q were qualitatively explained by using mean-field classical transport theory based on a classical-trajectory Monte Carlo simulation.

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高效率的电子冷却过程,要求电子束与离子束相互平行,要求电子束与离子束同轴。为了同时测量电子束与离子束的相对位置和夹角,考虑了容式、感式、条带型束流位置探针特点以及电子冷却段实际情况,在HIRFL-CSR电子冷却装置上建立了以容性圆筒形极板为感应电极、NI公司PXI-5105高精度数字化仪为数据采集设备、PET公司P/N AM-4A-000110-11030N型宽带放大器为信号处理电路的束流位置测量系统。通过测量束流通过探针时在极板上产生的脉冲信号,对其进行傅立叶变换得到频谱信号,分析四个不同电极上的频谱信号强度获取束流的位置信息。同时,为了调整电子束与离子束的相对位置和夹角,建立了一套以ADLINK公司的PCI-9113和PCI-6216数据卡为主,针对电子冷却装置中各螺线管电源、静电偏转板电源、校正线圈电源的控制系统,完成了校正线圈、静电偏转板以及螺线管对电子束位置的偏移、扫描,实现了电子束的位置、角度调整。 通过使用位置测量系统、电子束位置调整系统获得了校正线圈、螺线管、静电偏转板对电子束的位置偏移能力以及电子束的流强、电流密度分布、径向尺寸、绝热展开因子对束流位置的影响。在冷却累积过程中进行了改变电子束与离子束相对位置、夹角的实验,观察到了冷却力和离子束流强随相对位置、夹角的变化趋势,进而优化相对位置和夹角,实现高冷却效率。 根据实验数据分析了位置测量系统的系统误差来源和精度,提出了今后提高束流位置测量系统、调整系统稳定性、精确性而需要进行的工作;在此基础上使用测量系统、调整系统进行了电子束、离子束相对位置和角度对冷却效果的影响等电子冷却相关实验工作

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本文简要叙述了快重离子在固体材料,特别是聚合物材料中引起的强电子激发效应研究的基本理论、发展历史和研究现状。描述了在兰州重离子加速器上完成的25 MeV/u 86Kr离子辐照叠层聚对苯二甲酸乙二醇酯膜(PET)和聚碳酸酯(PC)膜的实验及结果分析。应用傅立叶红外变换光谱(FT-IR)及X-射线衍射分析(XRD)方法研究了在不同电子能损及不同注量辐照条件下,高能Kr离子在聚合物PET和PC潜径迹中引起的的损伤效应。结果表明:高能Kr离子在聚合物PET、PC膜引起的损伤主要是由于辐照引起的断键及键的重组产生的官能团的降解及非晶化过程,损伤截面存在电子能损阈值,且与官能团的结构有关。 对PET的傅立叶红外变换光谱分析结果给出,电子能损为7.25 keV/nm时,对应官能团吸收峰794 cm-1, 849 cm-1, 1021 cm-1, 1341 cm-1, 1410 cm-1, 1505 cm-1,的损伤截面半径分别为:3.63 nm, 4.70 nm, 4.58 nm, 3.54 nm, 5.17 nm, 5.32 nm。X-射线衍射分析结果表明,PET的非晶化转变截面随离子注量和电子能损的增大而增加,(100)衍射峰的相对强度I/I0随离子注量的增加而指数衰减,对应电子能损为6.62, 6.93, 7.25 keV/nm,其相应的非晶化半径分别为4.86, 5.64, 6.77 nm。 对PC的傅立叶红外变换光谱分析表明,当电子能损比较小,大多数官能团的红外吸收无明显变化,直到当辐照注量为2×1012 ions/cm2 且电子能损比较大时,其绝对吸收强度才发生明显的改变。电子能损为6.37 keV/nm 时,对应官能团吸收峰为519 cm-1, 605 cm-1, 724 cm-1, 1014 cm-1,其损伤截面分别为:13.12, 45.40, 50.21, 56.28 nm2

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目的 :IL - 2与金黄色葡萄球菌肠毒素A和B融合基因的克隆及表达。方法 :分别在金黄色葡萄球菌肠毒素A2 2 7Ala、B基因的两端克隆上两个酶切位点HindⅢ ,KpnⅠ。将IL - 2基因突变 ,设计一段linker使之分别与SEA2 2 7Ala和SEB相连并克隆到PET表达载体中 ,在大肠杆菌DH5α(DE3) -Pass中表达。结果 :表达的蛋白占总蛋白 15 %。结论 :IL - 2与金黄色葡萄球菌肠毒素A和B融合蛋白能在大肠杆菌中有效表达