964 resultados para Carotenoid Cleavage Dioxygenase
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利用3’和5' RACE、Uneven PCR等技术成功地从胡萝卜肉质根中分离了茄红素β-环化酶、茄红素ε.环化酶和辣椒红/辣椒玉红素合酶cDNA以及茄红素β一环化酶基因5’端上游的部分序列,并研究了它们在胡萝卜肉质根中的表达模式,对胡萝卜中类胡萝卜素代谢和积累的分子机制进行了探讨。 胡萝卜茄红素β--环化酶cDNA(DCLYC1)长2089bp,包含一个1515bp的开放阅读框架,所编码蛋白长505个氨基酸,其一级结构与番茄、烟草和辣椒等植物的茄红素β--环化酶高度同源。与农杆菌和夏噬孢欧文氏菌等微生物的茄红素环化酶相似性较差,但相互间有3个短小的同源区,且蛋白疏水模式也十分相似。茄红素β--环化酶在胡萝卜肉质根中的表达受品种和组织特异性的调控。在紫色的富含茄红素的“齐头红”胡萝卜肉质根中该基因的表达受到了强烈的抑制,相反,在橙色的富含β--和α--胡萝卜素的“CA201”胡萝卜肉质根中表达十分活跃。茄红素β--环化酶和八氢番茄红素合酶基因的表达在肉质根的韧皮部和木质部之间存在差异,在韧皮部中的表达强于木质部。类胡萝卜素生物合成基因的差异表达是造成不同胡萝卜品种和组织中积累的类胡萝卜素的种类和含量不同的原因。 对紫色品种和橙色品种的茄红素β--环化酶基因组DNA的PCR分析表明两者的基因组中均存在茄红素β一环化酶基因。为了探明茄红素β--环化酶基因在不同胡萝卜品种中差异表达的原因,利用Uneven pCR从胡萝卜基因组DNA中分离克隆了茄红素β--环化酶基因5’端上游部分序列。该DNA片段长1.7kb,3’端286bp区域与DCLYC1的5’端序列交叉重叠,在GenBank中没有找到相似的序列。在1294bp-1336bp位置串连着3个TATA盒,结构十分特殊,在TATA盒上游大约700bβ位置有2个CAAT盒。瞬间表达实验证明它具有启动子活性,可以指导GUS基因在胡萝卜肉质根、叶片和茎等组织中表达。然而,其表达模式却与茄红素B.环化酶基因的Northern杂交结果不同,主要在韧皮部和木质部交界的分生组织中表达,同时在紫色胡萝卜肉质根中其表达并没有受到抑制。这一片段可能还不是完整的胡萝卜茄红素β--环化酶基因启动子,缺少了调控基因进行品种和组织特异性表达的部分序列元件。因此,分离更长的胡萝卜茄红素环化酶基因5’端上游序列,将有助于揭示茄红素β一环化酶基因呈品种和组织特异性表达的分子机制。 所分离的胡萝卜辣椒红/辣椒玉红素合酶cDNA (DCCCS)长1744bp,包含一个长1476bp的开放阅读框架,所编码蛋白长492个氨基酸。与辣椒和柑桔CCS的氨基酸序列同源性分别为为76.6%和75.3%,与DCLYC1等其它植物茄红素β--环化酶的氨基酸序列同源性为63.9-67.4%。DCCCS的表达模式在两个不同颜色的品种之间十分相似,在肉质根韧皮部中强烈表达,而在木质部中表达明显受到了抑制。由于CCS与LYC-B高度同源,有人认为CCS可能具有茄红素环化酶活性,然而本研究结果表明,DCCCS虽然在紫色的齐头红胡萝卜肉质根韧皮部中强烈表达,却没有影响细胞中积累大量的茄红素,因此DCCCS即使具有茄红素环化酶作用,其活性也是极低的。 分离到的胡萝卜茄红素ε--环化酶cDNA片段(DCL YC-E)长1264bp,包含了完整的3’端,5’端尚不完整。按照引物LYCP1上的阅读框架进行翻译得到长385个氨基酸的肽链与莴苣、番茄和拟南芥LYC-E肽链相应区域的氨基酸序列高度同源,达80.5%以上,其中与莴苣茄红素ε--环化酶最为接近。与拟南芥茄红素ε--环化酶第448位基团和莴苣茄红素ε--环化酶第457位基团对应的氨基酸基团为H。这一基团是一个分子开关,决定茄红素ε--环化酶是催化茄红素的一端还是两端形成ε--环,因此,胡萝卜茄红素ε--环化酶可能与莴苣茄红素ε--环化酶具有相同的功能,即可以催化对称的线性茄红素的两端均形成ε--环,生成双ε--环胡萝卜素。DCLYC-E在胡萝卜肉质根中表达模式与DCLYCI不同,在紫色品种齐头红肉质根韧皮部中表达十分强烈,没有受到抑制,而且明显强于木质部;在橙色品种CA201中DCLYCE的表达模式与DCLYCI相似,韧皮部中表达强,而木质部中相对弱得多。DCL YC-E的表达模式在所测试品种间没有差异。在富含茄红素的齐头红胡萝卜肉质根中DCL YC-E强烈表达,可见它并没有将茄红素大量转化为双ε--环胡萝卜素,因此该酶的功能和活性有待进一步研究。
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盐角草(Salicornia europaea L.)是一种叶片退化而茎肉质化,不具有盐腺和盐囊泡的真盐生植物,可以在1020 mM NaCl下生存。其特殊的形态适应特点使其成为研究植物抗盐性的良好实验材料。但目前与盐角草抗盐机理相关的生理和分子方面的研究还非常有限。本文以盐角草为材料,首先探讨了盐分和渗透胁迫对其光合作用和渗透平衡的影响,在此基础上进一步克隆了盐角草类胡萝卜素合成途径中的两个关键酶,八氢番茄红素合成酶(SePSY)和番茄红素β-环化酶(SeLCY)基因,并进行了功能分析。该研究对于了解类胡萝卜素在植物抗盐性中所起的作用具有重要意义。 盐分和渗透胁迫对其光合作用和渗透平衡影响的实验结果表明:200 mM NaCl是盐生植物盐角草生长的最适盐浓度,在该盐度下盐角草中叶绿素a/b的比值和光饱和点升高,植株的光合作用表现出增强的效应,植株生长最佳。而27% PEG-6000所模拟的渗透胁迫显著降低了盐角草中叶绿色a/b的比值,抑制其光合作用和生长。200 mM NaCl下,Na+的含量显著增加,但脯氨酸含量保持不变,说明Na+对盐角草渗透平衡的作用要强于脯氨酸。同时盐角草中液泡H+-ATPase(V-H+-ATPase)活性增强,而盐角草Na+/H+逆向转运蛋白基因(SeNHX1)在盐分和渗透胁迫下却表现为组成型表达;我们因此推断在盐分胁迫下,Na+的吸收是由于液泡H+-ATPase活性的增强,而不是诱导SeNHX1基因的表达。同时Na+的吸收可能进一步诱导了与光合作用相关基因的表达。 盐分对植物的影响涉及植物体内包括光合作用和活性氧代谢在内的多个代谢过程。在植物中,类胡萝卜素是植物捕光天线复合体(LHC)和光系统反应中心叶绿素结合蛋白的重要组成部分。植物体内类胡萝卜素能够清除植物叶绿体,线粒体和过氧化物体在电子传递过程中产生的活性氧。同时类胡萝卜素是植物激素ABA的前体。200 mM NaCl虽然增加了盐角草细胞的渗透势,但并没有对其造成氧化胁迫和离子毒害,相反提高了其光合能力。类胡萝卜素作为植物活性氧的淬灭剂和光系统的组成成分,可能在盐角草抗盐机理中发挥着比较重要的作用。在过去的十年中,类胡萝卜素研究大多集中在其生物合成和提高作物中类胡萝卜素含量方面,可是,在植物对非生物逆境(如氧化和盐分胁迫)的适应机制中,类胡萝卜素合成途径究竟发挥什么作用目前还不是很清楚。为了了解盐角草中类胡萝卜素合成途径在植物逆境的适应机制中所发挥的作用,本文采用RACE的方法克隆了盐角草类胡萝卜素合成途径中的两个关键酶基因 SePSY和SeLCY,将它们构建到植物表达载体SN1301中,转化拟南芥,并对它们进行了初步的功能分析。 研究发现盐角草SePSY基因全长1655 bp,编码419个氨基酸,推测分子量为47.2 kDa,等电点为8.92。其蛋白在1-65个氨基酸处有一个信号肽。在1-19和242-264氨基酸处有2个跨膜区。盐角草SeLCY基因全长1937 bp,编码498个氨基酸,推测分子量为56.1 kDa,等电点为8.41。其蛋白在1-37个氨基酸处有一个信号肽。在79-96,367-385和454-474氨基酸处有3个跨膜区。SePSY和SeLCY基因过量表达均促进转基因拟南芥的生长,转SePSY基因拟南芥次生根数目比野生型拟南芥明显增多。SePSY和SeLCY基因的过量表达还使转基因拟南芥对百草枯的抗性得到提高;SePSY基 因的过量表达增强了植株体内抗氧化保护酶过氧化物酶(POD),超氧化物歧化酶(SOD)活性,但过氧化氢酶 (CAT)的变化不显著;转SeLCY基因株系POD,SOD,CAT的活性都有所增强,但转SePSY基因株系中POD活性明显高于 转SeLCY基因株系。转SePSY和SeLCY基因拟南芥叶片中丙二醛(MDA)和H2O2含量均降低,但转SePSY基因株系中MDA和H2O2含量明显低于转SeLCY基因株系。说明转基因拟南芥对氧化胁迫的抗性得到了提高,同时使得光系统II(PSII)和细胞膜的结构和功能不被破坏。而转SePSY基因株系对盐分和氧化胁迫的抗性明显高于转SeLCY基因株系。SePSY和SeLCY基因的过量表达还提高了转基因拟南芥的光合效率,气孔导度和Fv/Fm比值。 SePSY和SeLCY基因转化拟南芥及其功能分析的初步结果表明,SePSY和SeLCY基因的过量表达提高了转基因拟南芥对体内活性氧(ROS)的清除能力,增强了拟南芥的光合能力,进而提高了拟南芥的抗盐性。
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Fish flour from dried waste consisting of head, tail, fins and entrails was enzimatically hydrolysed using various proteases and the hydrolysate was spray dried. The functional properties such as water-fat absorption ratio, foaming and solubility index of the hydrolysates and fish flour revealed that some of the products might find significant uses in the food and/or cosmetics industry. Electrophoretic separation of the proteins from the fish flour and of the hydrolysates indicated that almost all the flour proteins are susceptible to proteolytic cleavage with the exception of one or two. The extent of degree of hydrolysis from 43-70.3% with a simultaneous decrease in unpleasant smell suggest an economical tool for minimizing odour pollution due to fish industry waste deterioration.
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Human ingenuity has made it possible to advent the chromosome manipulation techniques to produce individuals with differing genomic status in a number of fish using various causal agents such as physical shocks (temperature or hydrostatic pressure), chemical (endomitotics) and anesthetic treatments either to suppress the second meiotic division shortly after fertilization of eggs or to prevent the first mitotic division shortly prior to mitotic cleavage formation. This results in the induction of polyploidy (triploidy and tetraploidy), gynogenesis (both meiotic and mitotic leading to clonal lines) and androgenesis in fish population. The rationale for the induction of such ploidy in fish has been its potential for generating sterile individuals, rapidly inbred lines and masculinized fish, which could be of benefit to fish farming and aquaculture. In this paper, these are critically reviewed and the implication of recently developed chromosome manipulation techniques to various fin fishes is discussed.
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盐胁迫是限制高等植物和藻类生长和产量的主要环境因子之一。PSII对环境胁迫的响应被认为是光合作用适应逆境过程中最重要的一个环节。尽管盐胁迫对PSII的影响已进行了大量的研究,但有关盐胁迫对PSII作用方式和位点的研究仍存在着争议。我们主要研究了盐胁迫对螺旋藻PSII结构和功能的影响,以探讨盐胁迫对PSII的作用方式和位点以及该藻细胞PSII对盐胁迫的适应机理。主要研究结果如下: 1. 用0、0.2、0.4、0.6、0.8M NaCl处理螺旋藻细胞12小时。随盐浓度的增加,螺旋藻细胞的Chla、carotenoid、PC、APC及蛋白含量均呈下降趋势,说明盐胁迫抑制了上述色素及蛋白的合成或加速了它们的降解,从而影响了螺旋藻的光合作用。 2. 随盐浓度的增加,螺旋藻细胞光合放氧活性和PS II电子传递活性显著降低,表明盐胁迫引起藻细胞PS II活性的下降。 3. 通过放氧活性、热致发光(TL)、多相荧光瞬态上升动力学曲线的测定以及Western 杂交,来探讨盐胁迫对螺旋藻细胞PS II供体侧电子传递及OEC33蛋白含量的影响。结果显示:随盐浓度的增加,螺旋藻细胞光合放氧活性和PS II电子传递活性下降;TL B-band和Q-band强度降低,在0-0.6M NaCl下,B-band的周期性振荡清楚,最大值出现在第二次和第六次闪光,而在0.8M NaCl时,S态振荡基本上消失,S 态氧化还原循环受阻;Fm, J、I和P相荧光水平降低。以上结果都表明盐胁迫使PS II的放氧侧受损伤。且随盐浓度的增加,盐分引起螺旋藻细胞外周蛋白OEC33的降解,在蓝藻中首次提出放氧机构的S态循环受阻,放氧活性降低。 4. 通过OJIP曲线的测定以及JIP-test、闪光诱导的可变荧光衰减动力学、热致发光(TL)的分析,我们研究了盐胁迫对螺旋藻细胞PS II受体侧的影响。结果显示: JIP-test的参数Ψo和φEo随盐浓度的增加而下降,显示QA-到QB 电子传递受阻;可变荧光衰减动力学快相组分半衰期延长,所占总可变荧光百分比下降,表明QA-到QB 电子转移变慢,中相组分半衰期延长、所占百分比下降,说明空的QB位点对PQ的结合减慢,有可能PQ分子对QB位点的结合能力下降;TL B-band和Q-band的峰温度出现了位移,可能QA、QB的氧化还原电势发生了改变。以上结果表明,盐胁迫伤害了PSII受体侧的电子传递。 5. 首次运用闪光诱导下的叶绿素荧光上升及其衰减动力学来研究盐胁迫对PS II受体侧的影响。 6. 盐胁迫下,PS II供体侧和受体侧电子传递受抑制,有活性的PSII反应中心数量下降,说明盐胁迫对螺旋藻细胞PSII的伤害也可能是多位点的作用方式。此外,盐胁迫下,藻细胞放氧活性的下降快于受体侧QA 到QB电子传递所占百分比的下降,有可能PS II放氧侧先受损伤,然后是反应中心和受体侧。上述结果表明盐胁迫下PSII活性的降低是由于PSII供体侧和受体侧电子传递的抑制,有活性的PSII反应中心的减少。 7. 借助螺旋藻类囊体膜的Western杂交分析,来研究盐胁迫对螺旋藻类囊体膜PSII相关蛋白的影响。结果表明,上述PSII活性的抑制是由于类囊体膜蛋白的损失。主要与PSII反应中心CP43、CP47和OEC33蛋白含量的下降有关。 8. PS II机构对盐胁迫的适应涉及以下几个方面:降低吸收横截面,(PC/chla,APC/chla比值的降低);光系统II光化学反应的改变,通过关闭的PS II反应中心比例的增加,使得PS II机构免于过多激发能的伤害而得以保护;提高了剩余的有活性反应中心的耗能效率(DIo/RC增加);保持有活性反应中心高的激发能转化效率,比如,TRo/RC保持不变;另外,随盐浓度的增加,由藻胆体向光系统I的能量传递增加,避免过量激发能对 PSII的伤害,使螺旋藻细胞适应盐胁迫环境。
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Predictions for a 75x205mm surface semi-elliptic defect in the NESC-1 spinning cylinder test have been made using BS PD 6493:1991, the R6 procedure, non-linear cracked body finite element analysis techniques and the local approach to fracture. All the techniques agree in predicting ductile tearing near the inner surface of the cylinder followed by cleavage initiation. However they differ in the amount of ductile tearing, and the exact location and time of any cleavage event. The amount of ductile tearing decreases with increasing sophistication in the analysis, due to the drop in peak crack driving force and more explicit consideration of constraint effects. The local approach predicts a high probability of cleavage in both HAZ and base material after 190s, while the other predictions suggest that cleavage is unlikely in the HAZ due to constraint loss, but likely in the underlying base material. The timing of this event varies from ∼150s for R6 predictions to ∼250-300s using non-linear cracked body analysis.
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MicroRNAs (miRNAs) are a growing class of small RNAs ( about 22 nt) that play crucial regulatory roles in the genome by targeting mRNAs for cleavage or translational repression. Most of the identified miRNAs are highly conserved among species, indicating
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In order to study the early developmental stages of Nandus nandus an experiment was conducted, where eggs and milt were obtained from the laboratory reared N nandus by stripping after 15 hours of 150 mg/kg body weight of carp PG extract injection. Then the eggs were fertilized in the laboratory and subsequent developmental stages were studied. First cleavage (two cell), four cell, eight cell, sixteen cell and multi cell stages were found 30, 50, 70, 105 and 160 minutes after fertilization respectively. Morula, early gastrula, middle gastrula, late gastrula and yolk plug stages were found 5, 8, 9, 11 and 13 hours after fertilization respectively. Hatching occurred within 20±2 hours after fertilization, and larvae were measured 1.60 mm in diameter. After one hour of hatching two melanophore bands were found at the caudal region of the body of the larvae. Eyes were first observed in l 0 hours, pectoral and pelvic fin buds appeared in 22 hours and well developed in 38 hours old larvae. Mouth cleft and brain lobes were visible when the larvae were 34 and 38 hours old respectively. Myomeres partially appeared in 16 hours, which were clearly visible in 74 hours old larvae. Larvae started wandering and searching for food after 56 hours of hatching. The yolk sac was completely absorbed when larvae became 62 hours old.
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A novel plasminogen activator from Trimeresurus stejnegeri venom (TSV-PA) has been identified and purified to homogeneity. It is a single chain glycoprotein with an apparent molecular weight of 33,000 and an isoelectric point of pH 5.2. It specifically activates plasminogen through an enzymatic reaction. The activation of human native GIu-plasminogen by TSV-PA is due to a single cleavage of the molecule at the peptide bond Arg(561)-Val-(562). Purified TSV-PA, which catalyzes the hydrolysis of several tripeptide p-nitroanilide substrates, does not activate nor degrade prothrombin, factor X, or protein C and does not clot fibrinogen nor show fibrino(geno)lytic activity in the absence of plasminogen. The activity of TSV-PA was readily inhibited by phenylmethanesulfonyl fluoride and by p-nitrophenyl-p-guanidinobenzoate. Oligonucleotide primers designed on the basis of the N-terminal and the internal peptide sequences of TSV-PA were used for the amplification of cDNA fragments by polymerase chain reaction. This allowed the cloning of a full-length cDNA encoding TSV-PA from a cDNA library prepared from the venom glands. The deduced complete amino acid sequence of TSV-PA indicates that the mature TSV-PA protein is composed of 234 amino acids and contains a single potential N-gIycosylation site at Asn(1G1). The sequence of TSV-PA exhibits a high degree of sequence identity with other snake venom proteases: 66% with the protein C activator from Aghistrodon contortrix contortrix venom, 63% with batroxobin, and 60% with the factor V activator from Russell's viper venom. On the other hand, TSV-PA shows only 21-23% sequence similarity with the catalytic domains of u-PA and t-PA. Furthermore, TSV-PA lacks the sequence site that has been demonstrated to be responsible for the interaction of t-PA (KHRR) and u-PA (RRHR) with plasminogen activator inhibitor type 1.
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Amphibian skin contains rich neuropeptides. In the present study, a novel neuromedin U (NmU) analog was isolated from skin secretions of Chinese red belly Load Bombina maxima. Being 17-amino acids long, its primary structure was established as DSSGIVGRPFFLFRPRN-NH2, in which the C-terminal 8-residue segment (FFLFRPRN) is the same as that of rat NmU, while the N-terminal part DSSGIVGRP shows a great sequence variation compared with those of NmU peptides from different resources. The peptide, named Bm-NmU-17, was found to elicit concentration-dependent contractile effects on smooth muscle of rat uterus horns. The cDNA Structure of the peptide, as obtained by a 3'-RACE strategy and subsequently cloning from a skin cDNA library, was found to contain a coding region of 438 nucleotides. The encoded precursor is composed of 145 amino acids with a single copy of Bm-NmU-17 located towards the C-terminus. The sequence of the peptide is preceded by a dibasic site (Lys-Arg) and followed by the sequence of Gly-Arg-Lys, providing the sites of cleavage and releasing of the mature peptide. (c) 2005 Elsevier B.V. All rights reserved.
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Anabarilius grahami is a cyprinoid fish endemic to Fuxian Lake, Yunnan, China. In this study, a comprehensive staging series of A. grahami was produced. The embryonic development of A. grahami was divided into six main periods: zygote period, cleavage per
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Two different forms of Chinese pangolins can be recognized according to the color of their scales, i.e., brown and dusky. We analyzed mitochondrial DNA (mtDNA) purified from the livers of seven dusky and six brown Chinese pangolins from the same locality, using cleavage patterns from 19 restriction enzymes. From the 19 6-bp recognition enzymes used, 51-56 sites were observed. By combining the cleavage patterns for each enzyme, the 13 samples were classified into four restriction types: two in dusky and two in brown Chinese pangolins. The estimated number of nucleotide substitutions per site in dusky and brown types is 0.002, and that between dusky and brown types is 0.012. Divergence between brown and dusky forms began 0.6 Myr ago, provided the mean rate of sequence divergence is 0.02 per Myr in mtDNA. Our results suggest that there is considerable divergence in Chinese pangolins, and brown and dusky Chinese pangolins may be quite different forms or, at least, belong to different maternal groups.
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Mitochondrial DNA, purified from 36 samples of 23 local populations which are widely distributed in Vietnam, Burma, and 10 provinces of China, has been analyzed to model the phylogeny of rhesus monkeys. The 20 local populations of China may represent nearly all major populations in China. Using 20 restriction endonucleases of 6-bp recognition, we observed a total of 50-61 sites in the various samples. By combining the cleavage patterns for each enzyme, the 36 samples were classified into 23 restriction types, each of which was found exclusively in the respective population from which samples were obtained By combining the earlier study of Indian rhesus monkeys, phylogenetic trees, which have been constructed on the basis of genetic distance, indicate that rhesus monkeys in China, Vietnam, India, and Burma can be divided into seven groups. Integrating morphological and geographical data, we suggest that rhesus monkeys in China, Vietnam, and Burma may be classified into six subspecies-M. m. mulatta, M. m. brevicaudus, M. m. lasiotis, M. m. littoralis, M. m. vestita, and M. m. tcheliensis-and rhesus monkeys in India may be another valid subspecies. M. m. tcheliensis is the most endangered subspecies in China. Divergence among subspecies may have begun 0.9-1.6 Ma. The radiation of rhesus monkeys in China may have spread from the southwest toward the east. The taxonomic status of the Hainan monkey and the Taiwan monkey require further investigation.
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Mitochondrial DNAs (mtDNAs) purified from 25 samples of 6 species of macaques, Macaca mulatta, M. fascicularis, M. arctoides, M. nemestrina, M. assamensis and M. thibetana, were analyzed to study the phyletic relationships among the species. A total of 36-46 sites was observed in each sample. By combining the cleavage patterns for each of the endonucleases, the 25 samples were classified into 11 restriction types. When data on M. fuscata and M. cyclopis collected by other authors were added to our own, the resultant molecular phylogenetic trees indicated that the 8 species may be divided into 4 groups: (1) M. mulatta, M. fuscata, M. cyclopis and M. fascicularis; (2) M. arctoides, (3) M. nemestrina; (4) M. assamensis and M. thibetana. Our results suggest that within both the fascicularis and sinica groups genetic distances are small between members and that the status of the species within the groups may require further investigation.
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Bone marrow-derived mesenchymal stem cells (MSCs) hold great promise for treating immune disorders because of their immunoregulatory capacity, but the mechanism remains controversial. As we show here, the mechanism of MSC-mediated immunosuppression varies
