SDHA与肿瘤细胞代谢

细胞之间的营养竞争可以影响细胞的生长、生存和功能,不同的细胞对营养摄取条件不同,能量代谢表型各有差异,因此,细胞的状态与能量代谢是密切相关的.琥珀酸脱氢酶(SDH)位于线粒体内膜,是三羧酸循环的本质.SDH基因的突变与多种肿瘤有关.线粒体琥珀酸脱氢酶复合体是由多个亚基构成,包括SDHA、SDHB、SDHC、SDHD.其中SDHA扮演着重要的角色,SDHA突变可以引起SDH肿瘤组织中的酶活性丢失.免疫组织化学和转录组分析表明,SDHA突变会引起假性缺氧,导致血管生成增加,及其他SDHx基因突变.线粒体琥珀酸脱氢酶复合体亚单位A(SDHA)同时为线粒体电子传递链提供电子.SDHA的异常表达在肿瘤发生的过程中起到关键作用.本文从SDHA影响肿瘤细胞中能量代谢出发,对SDHA进行综述.     

辣椒雄性不育系SDH4基因的表达特性分析

为了探究线粒体电子传递复合体Ⅱ的关键酶基因(SDH4)与辣椒细胞质雄性不育的关系,该试验通过GenBank报道的辣椒线粒体基因组序列,特异引物扩增SDH4基因,并通过分析SDH4基因的时空表达及转录本编辑位点,以期找到辣椒细胞质雄性不育系9704A和保持系9704B的差异。结果表明:(1)从辣椒细胞质雄性不育系9704A和保持系9704B中获得的目的基因编码区片段长度一致,全长均为378bp,编码125个氨基酸残基。(2)辣椒保持系不同组织中SDH4基因表达存在差异,种子中表达最高,茎中表达最低。(3)在不同材料花蕾发育的同一时期,SDH4基因表达也不一致,在花粉母细胞减数分裂时期,不育系SDH4基因表达量明显低于保持系;而在造孢细胞增殖期、小孢子单核期和小孢子成熟期的表达量均高于保持系。(4)不育材料中SDH4基因在29位点出现RNA编辑,导致氨基酸由丝氨酸变为亮氨酸,增强了蛋白结构的疏水性能。研究认为,辣椒细胞质雄性不育系9704A和保持系9704B中SDH4基因的表达差异可能引起植物的能量代谢供应出现异常,从而导致雄性不育的产生。     

MUC1及其C端活性片段突变体具有抑制肿瘤的活性

MUC1蛋白翻译后成为一条多肽链,它很快在内质网被切割成2个亚基,形成稳定的异源二聚体.Cys-Gln-Cys(CQC)3个氨基酸位于MUC1C端亚基跨膜结构域与胞内结构域的连接处.研究发现,MUC1C端的CQCRRK结构域突变成AQARRK或使其缺失,突变体的致瘤性明显降低.表明:通过突变CQC→AQA来阻碍与C端亚基相关的二聚体化,可能成为肿瘤治疗的新途径.     

钠离子通道β4亚基糖基化的初步研究

异常表达的糖蛋白与PD等多种神经退行性疾病有关。糖蛋白组学研究发现,电压门控钠离子通道β4亚基在PD病人脑组织中表达明显增加。为了深入探索β4亚基及其糖链在帕金森发生发展中的作用,采用PD转基因鼠对其表达进行验证,对其潜在的糖基化位点进行定点突变,构建重组表达质粒。结果发现,在新生PD转基因鼠和野生成鼠脑组织中有~38kDa蛋白条带表达,而在新生野生鼠脑组织中不表达;用PNGase F酶处理去除糖链后,~38kDa蛋白条带变成迁移速递更快的较小分子量条带,说明β4亚基是高度糖基化的蛋白,并且其糖基化与生长发育有关。将突变重组质粒转入HEK-293细胞和小鼠神经瘤细胞Neuro2A中表达,结果发现突变型质粒分子量明显低于野生型。为研究β4亚基及其糖链的功能提供了一定的实验数据并打下了基础。     

白菜CesA基因家族鉴定及表达模式分析

为探究CesA基因家族在白菜生长发育及纤维素合成过程中的作用机制,该文通过生物信息学的方法,以白菜的全基因组序列为研究区域,进行理化特征、基因结构、进化特征、保守基序及结构域、顺式作用元件和组织表达等鉴定分析。结果表明:(1)共鉴定出16个编码纤维素合成酶亚基的CesA基因,该家族成员所编码蛋白的理论等电点为4.76～9.12,相对分子量为17.76～122.67 kD,长度为153～1 089 aa。(2)15个基因不均匀地分布于白菜的7条染色体上,Bra036008定位于scaffold上。(3)大部分成员包含4～14个外显子,1～11个保守基序。(4)该家族具有保守的DDD-QXXRW 保守功能域。(5)该家族编码蛋白主要分布在质膜上,二级结构以无规则卷曲与α-螺旋为主,多数成员都含有CesA蛋白典型的N端、C端和跨膜区。(6)CesA基因在茎中表达量相对较高,其中Bra011865、Bra023952和Bra029874在茎、叶、花中显著表达。该研究结果为后续深入研究CesA基因功能以及白菜生长发育研究奠定了基础。     

褪黑素通过减弱催乳素基因增强子的突变抑制大鼠垂体催乳素瘤的增生

本工作旨在探讨褪黑素(melatonin,MLT)抑制17-β-雌二醇(17-β-estradiol,E2)诱发的Sprague-Dawley大鼠垂体催乳素(prolactin,PRL)瘤增生的分子机制。结果表明,每只大鼠每日定时皮下注射一定剂量的MLT(0.25、0.50mg)能显著抑制E2诱发的大鼠垂体PRL瘤的增生;偏低(0.05mg)或过高剂量(1.00、2.00mg)的MLT也抑制PRL瘤的增生,但无统计学意义。采用PCR和DNA直接测序显示,与正常垂体对照组比较,PRL瘤中PRL基因增强子出现五处突变,-1885bp位点由C突变为G,-1857~-1855由ACA替换为G,-1792~-1791插入G,-1383~-1382插入GGTGTGTG片段,-1265~-1250缺失GTGTGTGTGTGTGTGT片段。0.25mg/dMLT处理组,PRL瘤中的PRL基因增强子上述个别突变部位仍然存在(-1885由C突变为G),突变消失(-1792~-1791无插入G),大部分表现为突变减弱(-1856~-1855缺失AC,-1385~-1384缺失TG,-1250~-1253缺失GTGT)。采用荧光素酶报告基因检测PRL基因增强子活性显示,正常垂体、PRL瘤和0.25mg/dMLT处理的PRL瘤三组中,PRL基因增强子的活性分别为(13448.17±3012.74)、(161831.67±60996.01)和(10212.17±2634.71)OD单位。PRL瘤组增强子活性较正常垂体升高11倍(P<0.001),MLT处理组增强子活性较PRL瘤组降低93.69%(P<0.001)。上述三组PRL基因增强子空间结构的分析表明,PRL基因增强子DNA的曲折程度为PRL瘤组>MLT处理组>正常垂体。以上结果证实,MLT抑制大鼠垂体PRL瘤增生的重要分子机制之一可能是减弱PRL基因增强子的突变,也提示MLT可减弱PRL基因增强子的突变,从而下调PRL基因的高表达,可能与降低DNA的曲折程度有关。     

拟南芥复制因子C亚基1在胚胎发生中起重要作用

复制因子C包含1个大亚基和4个小亚基,在DNA复制、损伤修复和细胞增殖中起重要作用,拟南芥复制因子C亚基1(AtRFC1)是人类复制因子C大亚基p140的同源蛋白。在对3个复制因子C亚基1的T-DNA插入突变株系rfc1-1、rfc1-2和rfc1-3的检验中,证实插入位点分别位于第16、19号外显子和启动子区域。T-DNA在外显子中的插入突变引起胚胎发育异常并导致胚胎和种子败育。将野生型拟南芥复制因子C亚基1基因转化到突变株系rfc1-1和rfc1-2后恢复了突变株的野生型表型,证明胚胎发生异常表型是由拟南芥复制因子C亚基1基因突变所引起的,AtRFC1在拟南芥胚胎发生中起重要作用。     

用差异显示反转录PCR银染技术研究植物基因表达的差异

通过调整差异显示反转录PCR(DDRT-PCR)中总RNA、锚定引物、随机引物、cDNA和dNTP等关键试剂的用量,优化了适用于银染检测的DDRT-PCR方法.PCR扩增产物经6%变性聚丙烯酰胺凝胶垂直电泳分离后,银染能检测到多而清晰的条带.泳道中的条带数最少为40个,最多达80个,平均为60个,条带大小分布在100～900 bp范围,灵敏度为5 pg/mm² .此方法操作简便快速,灵敏度高,重复性好.采用这个改良的方法,分析了拟南芥野生型和ast突变型基因表达的差异.从16 000个cDNA扩增产物条带中筛选出28个差异条带.二次PCR扩增后,进一步筛选出13个差异条带,其中7个是野生型特异表达的,6个是突变型特异表达的,为进一步认识ast突变表型的产生机制奠定了基础.     

老年痴呆症相关基因Nicastrin的转录调控

APP蛋白经过降解,形成老年痴呆症患者脑内老年斑的主要成分．由PS(早老素),NCT, PEN-2和APH-1 4种膜蛋白组成的γ分泌酶催化该降解过程．为了了解人类nicastrin( NCT )基因的转录调控机制,确定了其在人脑中的转录起始位点以及其编码区上游大小不等片段的转录起始活性．EMSA分析证实NCT启动子区的4个AP-1结合位点和2个NFAT结合位点能够与相应的转录因子结合,能够改变转录因子调控能力的定点突变和PDTC诱导使得NCT启动子在HeLa细胞和大鼠皮质神经元中的启动活性都有所改变．以上结果说明：AP-1和NFAT确实参与了人类NCT基因的转录调控．     

大瘤足蕨和镰羽瘤足蕨的化学成分研究

对瘤足蕨属中的大瘤足蕨和镰羽瘤足蕨进行化学成分研究,从这两种植物中分离并鉴定了9个化合物,分别是:大波斯菊苷(1)、异山奈甲黄素(2)、astragalin(3)、3β,27-dihydroxylup-12-ene(4)、hydroxyhopanone(5)、plagiogyrin a(6)、androsin(7)、β-谷甾醇(8)、β-胡萝卜苷(9).所有化合物均为首次从这两种植物中分离得到,其中化合物1、4、7、9为这两种植物的共有成分.     

Evolution of a secondary metabolic pathway from primary metabolism: shikimate and quinate biosynthesis in plants

The shikimate pathway synthesizes aromatic amino acids essential for protein biosynthesis. Shikimate dehydrogenase (SDH) is a central enzyme of this primary metabolic pathway, producing shikimate. The structurally similar quinate is a secondary metabolite synthesized by quinate dehydrogenase (QDH). SDH and QDH belong to the same gene family, which diverged into two phylogenetic clades after a defining gene duplication just prior to the angiosperm/gymnosperm split. Non‐seed plants that diverged before this duplication harbour only a single gene of this family. Extant representatives from the chlorophytes (Chlamydomonas reinhardtii), bryophytes (Physcomitrella patens) and lycophytes (Selaginella moellendorfii) encoded almost exclusively SDH activity in vitro. A reconstructed ancestral sequence representing the node just prior to the gene duplication also encoded SDH activity. Quinate dehydrogenase activity was gained only in seed plants following gene duplication. Quinate dehydrogenases of gymnosperms, represented here by Pinus taeda, may be reminiscent of an evolutionary intermediate since they encode equal SDH and QDH activities. The second copy in P. taeda maintained specificity for shikimate similar to the activity found in the angiosperm SDH sister clade. The codon for a tyrosine residue within the active site displayed a signature of positive selection at the node defining the QDH clade, where it changed to a glycine. Replacing the tyrosine with a glycine in a highly shikimate‐specific angiosperm SDH was sufficient to gain some QDH function. Thus, very few mutations were necessary to facilitate the evolution of QDH genes.     

Pulsed EPR investigations of the Mo(V) centers of the R55Q and R55M variants of sulfite dehydrogenase from Starkeya novella

Continuous-wave and pulsed electron paramagnetic resonance (EPR) spectroscopy have been used to characterize two variants of bacterial sulfite dehydrogenase (SDH) from Starkeya novella in which the conserved active-site arginine residue (R55) is replaced by a neutral amino acid residue. Substitution by the hydrophobic methionine residue (SDH^R55M) has essentially no effect on the pH dependence of the EPR properties of the Mo(V) center, even though the X-ray structure of this variant shows that the methionine residue is rotated away from the Mo center and a sulfate anion is present in the active-site pocket (Bailey et al. in J Biol Chem 284:2053–2063, 2009). For SDH^R55M only the high-pH form is observed, and samples prepared in H₂ ¹⁷O-enriched buffer show essentially the same ¹⁷O hyperfine interaction and nuclear quadrupole interaction parameters as SDH^WT enzyme. However, the pH dependence of the EPR spectra of SDH^R55Q, in which the positively charged arginine is replaced by the neutral hydrophilic glutamine, differs significantly from that of SDH^WT. For SDH^R55Q the blocked form with bound sulfate is generated at low pH, as verified by ³³S couplings observed upon reduction with ³³S-labeled sulfite. This observation of bound sulfate for SDH^R55Q supports our previous hypothesis that sulfite-oxidizing enzymes can exhibit multiple pathways for electron transfer and product release (Emesh et al. in Biochemistry 48:2156–2163, 2009). At pH ≥ 8 the high-pH form dominates for SDH^R55Q.     

Mutations in the C. elegans Succinate Dehydrogenase Iron-Sulfur Subunit Promote Superoxide Generation and Premature Aging

The mitochondrial succinate dehydrogenase (SDH) is an iron-sulfur flavoenzyme linking the Krebs cycle and the mitochondrial respiratory chain. Mutations in the human SDHB, SDHC and SDHD genes are responsible for the development of paraganglioma and pheochromocytoma, tumors of the head and neck or the adrenal medulla, respectively. In recent years, SDH has become recognized as a source of reactive oxygen species, which may contribute to tumorigenesis. We have developed a Caenorhabditis elegans model to investigate the molecular and catalytic effects of mutations in the sdhb-1 gene, which encodes the SDH iron-sulfur subunit. We created mutations in Pro211; this residue is located near the site of ubiquinone reduction and is conserved in human SDHB (Pro197), where it is associated with tumorigenesis. Mutant phenotypes ranged from relatively benign to lethal and were characterized by hypersensitivity to oxidative stress, a shortened life span, impaired respiration and overproduction of superoxide. Our data suggest that the SDH ubiquinone-binding site can become a source of superoxide and that the pathological consequences of SDH mutations can be mitigated with antioxidants, such as ascorbate and N-acetyl-l-cysteine. Our work leads to a better understanding of the relationship between genotype and phenotype in respiratory chain mutations and of the mechanisms of aging and tumorigenesis.     

Cloning of cDNAs encoding sorbitol dehydrogenase-2a and b, enzymatic characterization, and up-regulated expression of the genes in Bombyx mori diapause eggs exposed to 5 °C

We previously cloned a cDNA for sorbitol dehydrogenase (SDH1) from Bombyx mori. In the present study we cloned two additional cDNAs encoding SDHs (designated as SDH2a and SDH2b). The amino acid sequences of SDH2ab were almost the same and had higher similarity to the SDHs of other organisms than to B. mori SDH1. The SDH2ab and SDH1genes were located in tandem within about 40 kbp on chromosome 21. SDH2ab mRNAs increased after exposing diapause eggs to 5 °C for 40 days, beginning at 2 days post-oviposition, to break diapause. However, they were at very low levels in diapausing eggs incubated at 25 °C continuously from oviposition. These changes in expression pattern of SDH2ab mRNA were almost the same as that of SDH1 mRNA. To understand whether SDH1 and SDH2 were responsible for the SDH activity seen in diapause eggs exposed to 5 °C for more than 60 days, we expressed a His-tagged SDH2a fusion protein in Escherichia coli and examined its enzymatic parameters. The maximum activity of SDH2a observed at pH 8.4∼9.0, and the Km value for sorbitol was 12.6 mM, similar to the kinetic properties of other SDHs. Due to the significantly higher similarity between SDH2a and b, they were thought to have similar kinetic properties. Therefore, we purified SDH from B. mori diapause-terminated eggs exposed to 5 °C for 300 days which showed higher SDH activity using two-step affinity chromatography. The highly purified SDH showed a higher Km value (125 mM) for sorbitol, being similar to the value (136 mM) determined previously from Eadie-Hofstee plots using egg crude extract as an enzyme source; additionally, the plots showed one slope indicating one Km value. Moreover, in silico analysis indicated that no SDH genes other than SDH1 and 2ab are present in B. mori genomic DNA. These results suggest that SDH1 activity may be responsible for the majority of the increased SDH activity seen in diapause eggs after acclimation to 5 °C rather than SDH2ab. Further, the relative sequence divergence among these genes is consistent with the idea/hypothesis that the original SDH gene was first duplicated into SDH1 and SDH2, and then SDH2 was duplicated into the SDH2a and SDH2b genes.     

Molecular Characterization of Quinate and Shikimate Metabolism in Populus trichocarpa

The shikimate pathway leads to the biosynthesis of aromatic amino acids essential for protein biosynthesis and the production of a wide array of plant secondary metabolites. Among them, quinate is an astringent feeding deterrent that can be formed in a single step reaction from 3-dehydroquinate catalyzed by quinate dehydrogenase (QDH). 3-Dehydroquinate is also the substrate for shikimate biosynthesis through the sequential actions of dehydroquinate dehydratase (DQD) and shikimate dehydrogenase (SDH) contained in a single protein in plants. The reaction mechanism of QDH resembles that of SDH. The poplar genome encodes five DQD/SDH-like genes (Poptr1 to Poptr5), which have diverged into two distinct groups based on sequence analysis and protein structure prediction. In vitro biochemical assays proved that Poptr1 and -5 are true DQD/SDHs, whereas Poptr2 and -3 instead have QDH activity with only residual DQD/SDH activity. Poplar DQD/SDHs have distinct expression profiles suggesting separate roles in protein and lignin biosynthesis. Also, the QDH genes are differentially expressed. In summary, quinate (secondary metabolism) and shikimate (primary metabolism) metabolic activities are encoded by distinct members of the same gene family, each having different physiological functions.     

Three different genes encode the iron-sulfur subunit of succinate dehydrogenase in Arabidopsis thaliana

The iron-sulfur protein is an essential component of mitochondrial complex II (succinate dehydrogenase, SDH), which is a functional enzyme of both the citric acid cycle and the respiratory electron transport chain. This protein is encoded by a single-copy nuclear gene in mammals and fungi and by a mitochondrial gene in Rhodophyta and the protist Reclinomonas americana. In Arabidopsis thaliana, the homologous protein is now found to be encoded by three nuclear genes. Two genes (sdh2-1 andsdh2-2) likely arose from a relatively recent duplication event since they have similar structures, encode nearly identical proteins and show similar expression patterns. Both genes are interrupted by a single intron located at a conserved position. Expression was detected in all tissues analysed, with the highest steady-state mRNA levels found in flowers and inflorescences. In contrast, the third gene (sdh2-3) is interrupted by 4 introns, is expressed at a low level, and encodes a SDH2-3 protein which is only 67% similar to SDH2-1 and SDH2-2 and has a different N-terminal presequence. Interestingly, the proteins encoded by these three genes are probably functional because they are highly conserved compared with their homologues in other organisms. These proteins contain the cysteine motifs involved in binding the three iron-sulfur clusters essential for electron transport. Furthermore, the three polypeptides are found to be imported into isolated plant mitochondria.     

The driver and passenger effects of isocitrate dehydrogenase 1 and 2 mutations in oncogenesis and survival prolongation

Mutations in isocitrate dehydrogenase 1 and 2 (IDH1 and IDH2) are key events in the development of glioma, acute myeloid leukemia (AML), chondrosarcoma, intrahepatic cholangiocarcinoma (ICC), and angioimmunoblastic T-cell lymphoma. They also cause D-2-hydroxyglutaric aciduria and Ollier and Maffucci syndromes. IDH1/2 mutations are associated with prolonged survival in glioma and in ICC, but not in AML. The reason for this is unknown. In their wild-type forms, IDH1 and IDH2 convert isocitrate and NADP⁺ to α-ketoglutarate (αKG) and NADPH. Missense mutations in the active sites of these enzymes induce a neo-enzymatic reaction wherein NADPH reduces αKG to D-2-hydroxyglutarate (D-2HG). The resulting D-2HG accumulation leads to hypoxia-inducible factor 1α degradation, and changes in epigenetics and extracellular matrix homeostasis. Such mutations also imply less NADPH production capacity. Each of these effects could play a role in cancer formation. Here, we provide an overview of the literature and discuss which downstream molecular effects are likely to be the drivers of the oncogenic and survival-prolonging properties of IDH1/2 mutations. We discuss interactions between mutant IDH1/2 inhibitors and conventional therapies. Understanding of the biochemical consequences of IDH1/2 mutations in oncogenesis and survival prolongation will yield valuable information for rational therapy design: it will tell us which oncogenic processes should be blocked and which “survivalogenic” effects should be retained.     

Functional analysis through site-directed mutations and phylogeny of the Candida albicans LYS1-encoded saccharopine dehydrogenase

Candida albicans LYS1-encoded saccharopine dehydrogenase (CaLys1p, SDH) catalyzes the final biosynthetic step (saccharopine to lysine + α-ketoglutarate) of the novel α-aminoadipate pathway for lysine synthesis in fungi. The reverse reaction catalyzed by lysine-α-ketoglutarate reductase (LKR) is used exclusively in animals and plants for the catabolism of excess lysine. The 1,146 bp C. albicans LYS1 ORF encodes a 382 amino acid SDH. In the present investigation, we have used E. coli-expressed recombinant C. albicans Lys1p for the determination of both forward and reverse SDH activities in vitro, compared the sequence identity of C. albicans Lys1p with other known SDHs and LKRs, performed extensive site-directed mutational analyses of conserved amino acid residues and analyzed the phylogenetic relationship of C. albicans Lys1p to other known SDHs and LKRs. We have identified 14 of the 68 amino acid substitutions as essential for C. albicans Lys1p SDH activity, including two highly conserved functional motifs, H93XXF96XH98 and G138XXXG142XXG145. These results provided new insight into the functional and phylogenetic characteristics of the distinct biosynthetic SDH in fungi and catabolic LKR in higher eukaryotes.