Ectopic Gene Expression

异位基因表达
  • 文章类型: Journal Article
    结论:OsWOX9A的异位表达诱导狭窄的正面滚动水稻叶片,具有较大的球形细胞和较少的大静脉,可能通过调节生长素相关和expansin基因的表达。WUSCHEL相关同源异型盒(WOX)家族通过调节涉及生长和分化各个方面的基因,在植物发育中发挥关键作用。OsWOX9A(DWT1)与分till生长有关,植物生长均匀,和花分生组织活动。然而,其对水稻叶片生长发育的影响尚未研究。在这项研究中,我们使用转基因植物研究了OsWOX9A在水稻生长发育中的生物学作用。OsWOX9A的过度表达赋予了狭窄的正面滚动水稻叶片并改变了植物结构。与野生型植物相比,这些植物表现出较大的球形细胞和较少的较大静脉。OsWOX9A过表达也降低了株高,舵柄编号,和结实率。比较转录组分析揭示了OsWOX9A过表达植物中几个差异表达的生长素相关和expansin基因,与它们在叶片和植物发育中的作用一致。这些结果表明,OsWOX9A的异位表达可能对水稻的发育和生长有多重影响。更全面地了解WOX9亚科如何促进叶片发育和植物结构。
    CONCLUSIONS: Ectopic expression of OsWOX9A induces narrow adaxially rolled rice leaves with larger bulliform cells and fewer large veins, probably through regulating the expression of auxin-related and expansin genes. The WUSCHEL-related homeobox (WOX) family plays a pivotal role in plant development by regulating genes involved in various aspects of growth and differentiation. OsWOX9A (DWT1) has been linked to tiller growth, uniform plant growth, and flower meristem activity. However, its impact on leaf growth and development in rice has not been studied. In this study, we investigated the biological role of OsWOX9A in rice growth and development using transgenic plants. Overexpression of OsWOX9A conferred narrow adaxially rolled rice leaves and altered plant architecture. These plants exhibited larger bulliform cells and fewer larger veins compared to wild-type plants. OsWOX9A overexpression also reduced plant height, tiller number, and seed-setting rate. Comparative transcriptome analysis revealed several differentially expressed auxin-related and expansin genes in OsWOX9A overexpressing plants, consistent with their roles in leaf and plant development. These results indicate that the ectopic expression of OsWOX9A may have multiple effects on the development and growth of rice, providing a more comprehensive picture of how the WOX9 subfamily contributes to leaf development and plant architecture.
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  • 文章类型: Journal Article
    TGA结合(TGA)转录因子,以碱性区域/亮氨酸拉链基序(bZIP)为特征,被认为是植物生长的关键调节剂,发展,以及通过它们与as-1元素的结合而产生的应激反应。在这项研究中,甜瓜中的TGA基因家族,西瓜,黄瓜,南瓜,西葫芦的特征全面,包括基因/蛋白质结构的分析,系统发育关系,基因复制事件,和基因启动子中的顺式作用元件。在烟草中瞬时表达,甜瓜CmTGA,具有典型的bZIP和DOG1域,被观察到位于细胞核内。生化研究揭示了CmTGA2/3/5/8/9与CmNPR3或CmNPR4之间的特定相互作用。CmTGA基因在甜瓜植物中表现出差异表达模式,以响应不同的激素,如水杨酸,茉莉酸甲酯,和乙烯,以及真菌病原体,南瓜孢霉,引起甜瓜胶质茎枯病。CmTGA3,CmTGA8和CmTGA9在拟南芥植物中的过表达导致AtPR1和AtPR5表达上调,从而赋予对丁香假单胞菌pv的增强的抗性。番茄DC3000。相比之下,CmTGA7或CmTGA9的过表达导致对灰葡萄孢菌的抗性受损,与感染灰白杆菌后AtPDF1.2和AtMYC2的表达水平同时降低相吻合。这些发现揭示了特定CmTGA基因在植物免疫中的重要作用。表明对这些基因的遗传操作可能是增强植物免疫反应的有希望的途径。
    TGA-binding (TGA) transcription factors, characterized by the basic region/leucine zipper motif (bZIP), have been recognized as pivotal regulators in plant growth, development, and stress responses through their binding to the as-1 element. In this study, the TGA gene families in melon, watermelon, cucumber, pumpkin, and zucchini were comprehensively characterized, encompassing analyses of gene/protein structures, phylogenetic relationships, gene duplication events, and cis-acting elements in gene promoters. Upon transient expression in Nicotiana benthamiana, the melon CmTGAs, with typical bZIP and DOG1 domains, were observed to localize within the nucleus. Biochemical investigation revealed specific interactions between CmTGA2/3/5/8/9 and CmNPR3 or CmNPR4. The CmTGA genes exhibited differential expression patterns in melon plants in response to different hormones like salicylic acid, methyl jasmonate, and ethylene, as well as a fungal pathogen, Stagonosporopsis cucurbitacearum that causes gummy stem blight in melon. The overexpression of CmTGA3, CmTGA8, and CmTGA9 in Arabidopsis plants resulted in the upregulation of AtPR1 and AtPR5 expression, thereby imparting enhanced resistance to Pseudomonas syringae pv. Tomato DC3000. In contrast, the overexpression of CmTGA7 or CmTGA9 resulted in a compromised resistance to Botrytis cinerea, coinciding with a concomitant reduction in the expression levels of AtPDF1.2 and AtMYC2 following infection with B. cinerea. These findings shed light on the important roles of specific CmTGA genes in plant immunity, suggesting that genetic manipulation of these genes could be a promising avenue for enhancing plant immune responses.
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  • 文章类型: Journal Article
    磷酸烯醇丙酮酸羧化酶(PEPC)在C4植物的初始碳固定过程中起着至关重要的作用。然而,它在梭梭中的非光合功能,一种C4多年生干盐生灌木,仍然知之甚少。先前的研究报道了PEPC参与植物对非生物胁迫如干旱和盐胁迫的反应。然而,PEPC对干旱胁迫的耐受机制尚未确定。在这项研究中,我们从H.ammodendron中克隆了C4型PEPC基因HaPEPC1,并通过产生具有HaPEPC1异位表达的转基因拟南芥植物来研究其生物学功能。我们的研究结果表明,与WT(野生型)植物相比,HaPEPC1植物的异位表达显示出显着更高的发芽率和叶绿素含量。此外,在干旱胁迫下,转基因植物呈现增加的根长度,鲜重,光合能力,和抗氧化酶活性,特别是抗坏血酸过氧化物酶和过氧化物酶。此外,转基因植物的丙二醛水平降低,H2O2(过氧化氢),和O2-(超氧自由基)。转录组分析表明,HaPEPC1的异位表达主要调节与应激防御反应相关的基因的表达,谷胱甘肽代谢,以及响应干旱胁迫的脱落酸(ABA)合成和信号通路。一起来看,这些发现表明HaPEPC1的异位表达增强了转基因植物中H2O2和O2的减少,从而提高活性氧(ROS)清除能力,增强耐旱性。因此,HaPEPC1基因有望成为旨在增强耐旱性的作物选择的候选基因。
    Phosphoenolpyruvate carboxylase (PEPC) plays a crucial role in the initial carbon fixation process in C4 plants. However, its nonphotosynthetic functions in Haloxylon ammodendron, a C4 perennial xerohalophytic shrub, are still poorly understood. Previous studies have reported the involvement of PEPC in plant responses to abiotic stresses such as drought and salt stress. However, the underlying mechanism of PEPC tolerance to drought stress has not been determined. In this study, we cloned the C4-type PEPC gene HaPEPC1 from H. ammodendron and investigated its biological function by generating transgenic Arabidopsis plants with ectopic expression of HaPEPC1. Our results showed that, compared with WT (wild-type) plants, ectopic expression of HaPEPC1 plants exhibited significantly greater germination rates and chlorophyll contents. Furthermore, under drought stress, the transgenic plants presented increased root length, fresh weight, photosynthetic capacity, and antioxidant enzyme activities, particularly ascorbate peroxidase and peroxidase. Additionally, the transgenic plants exhibited reduced levels of malondialdehyde, H2O2 (hydrogen peroxide), and O2- (superoxide radical). Transcriptome analysis indicated that ectopic expression of HaPEPC1 primarily regulated the expression of genes associated with the stress defence response, glutathione metabolism, and abscisic acid (ABA) synthesis and signalling pathways in response to drought stress. Taken together, these findings suggest that the ectopic expression of HaPEPC1 enhances the reduction of H2O2 and O2- in transgenic plants, thereby improving reactive oxygen species (ROS) scavenging capacity and enhancing drought tolerance. Therefore, the HaPEPC1 gene holds promise as a candidate gene for crop selection aimed at enhancing drought tolerance.
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  • 文章类型: Journal Article
    在肌肉营养不良中,肌肉纤维松散的完整性和死亡,造成重大痛苦和过早死亡。引人注目的是,眼外肌(EOM)幸免,尽管疾病进展,但功能良好。尽管EOM已被证明与人体肌肉组织不同,这种对肌肉营养不良的固有抵抗力的潜在机制仍然未知。这里,我们通过转录组学分析证明了斑马鱼EOMs和躯干肌之间的基因表达对肌肉营养不良的反应的重要差异。我们表明LIM-蛋白Fhl2响应于desmin的敲除而增加,plectin和obsccurin,敲除导致不同肌肉营养不良的细胞骨架蛋白,并有助于EOM的疾病保护。此外,我们表明fhl2b的异位表达可以部分挽救斑马鱼Duchenne肌营养不良模型sapje的肌肉表型,显着提高他们的生存。因此,Fhl2是保护剂和用于治疗肌营养不良的候选靶基因。
    In muscular dystrophies, muscle fibers loose integrity and die, causing significant suffering and premature death. Strikingly, the extraocular muscles (EOMs) are spared, functioning well despite the disease progression. Although EOMs have been shown to differ from body musculature, the mechanisms underlying this inherent resistance to muscle dystrophies remain unknown. Here, we demonstrate important differences in gene expression as a response to muscle dystrophies between the EOMs and trunk muscles in zebrafish via transcriptomic profiling. We show that the LIM-protein Fhl2 is increased in response to the knockout of desmin, plectin and obscurin, cytoskeletal proteins whose knockout causes different muscle dystrophies, and contributes to disease protection of the EOMs. Moreover, we show that ectopic expression of fhl2b can partially rescue the muscle phenotype in the zebrafish Duchenne muscular dystrophy model sapje, significantly improving their survival. Therefore, Fhl2 is a protective agent and a candidate target gene for therapy of muscular dystrophies.
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  • 文章类型: Journal Article
    需要树木的初级和次级生长以增加植物高度和茎直径,分别,影响木材中木质生物质的生产,纸浆/纸,和相关的生物材料。这两种类型的生长被认为都受不同的转录因子(TF)介导的调节途径调节。值得注意的是,我们在毛果杨中鉴定了PtrLBD39,这是一种高度茎韧皮部特异性TF,并发现PtrLBD39在毛果杨中的异位表达显着阻碍了初级和次级生长。在这些过度表达的植物中,RNA-seq,ChIP-seq,和加权基因共表达网络分析(WGCNA)显示,PtrLBD39直接或间接调节调节血管组织发育的TFs,木材形成,激素信号通路,和负责木材成分的酶。这种调节导致生长抑制,纤维细胞次生细胞壁厚度减少,减少木材生产。因此,我们的研究表明,以下是毛果假单胞菌的异位表达,PtrLBD39充当影响初级和次级生长的阻遏物。
    Primary and secondary growth of trees are needed for increments in plant height and stem diameter, respectively, affecting the production of woody biomass for applications in timber, pulp/paper, and related biomaterials. These two types of growth are believed to be both regulated by distinct transcription factor (TF)-mediated regulatory pathways. Notably, we identified PtrLBD39, a highly stem phloem-specific TF in Populus trichocarpa and found that the ectopic expression of PtrLBD39 in P. trichocarpa markedly retarded both primary and secondary growth. In these overexpressing plants, the RNA-seq, ChIP-seq, and weighted gene co-expression network analysis (WGCNA) revealed that PtrLBD39 directly or indirectly regulates TFs governing vascular tissue development, wood formation, hormonal signaling pathways, and enzymes responsible for wood components. This regulation led to growth inhibition, decreased fibrocyte secondary cell wall thickness, and reduced wood production. Therefore, our study indicates that, following ectopic expression in P. trichocarpa, PtrLBD39 functions as a repressor influencing both primary and secondary growth.
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  • 文章类型: Journal Article
    染色体不稳定是骨髓增生异常综合征(MDS)的一个突出的生物学特征,超过50%的MDS患者具有染色体异常或复杂的核型。尽管有这样的观察,MDS有丝分裂和染色体缺陷的潜在机制仍然难以捉摸。在这项研究中,我们发现转录因子ONECUT3的异位表达与MDS的复杂核型和较差的生存结局相关.过表达ONECUT3的细胞模型显示出几个显著的途径的富集,包括姐妹染色体交换分离和有丝分裂核分裂的标志与INCENP和CDCA8基因的上调。值得注意的是,有丝分裂期除细胞赤道和中体外,染色体乘客复合物(CPC)积累的失调导致胞质分裂失败和染色体分离缺陷。机械上,ONECUT3的同源盒(HOX)域,作为DNA结合域,占据了INCENP和CDCA8的独特基因组区域,并转录激活了这两个基因。鉴定了一种新型先导化合物C5484617,该化合物在功能上靶向ONECUT3的HOX结构域,抑制其在下游基因上的转录活性,和协同性的再敏化MDS细胞对低甲基化剂。这项研究表明,ONECUT3通过INCENP和CDCA8的转录激活促进染色体不稳定性,提示靶向具有复杂核型的高危MDS患者的潜在预后和治疗作用。
    Chromosomal instability is a prominent biological feature of myelodysplastic syndromes (MDS), with over 50% of patients with MDS harboring chromosomal abnormalities or a complex karyotype (CK). Despite this observation, the mechanisms underlying mitotic and chromosomal defects in MDS remain elusive. In this study, we identified ectopic expression of the transcription factor ONECUT3, which is associated with CKs and poorer survival outcomes in MDS. ONECUT3-overexpressing cell models exhibited enrichment of several notable pathways, including signatures of sister chromosome exchange separation and mitotic nuclear division with the upregulation of INCENP and CDCA8 genes. Notably, dysregulation of chromosome passenger complex (CPC) accumulation, besides the cell equator and midbody, during mitotic phases consequently caused cytokinesis failure and defective chromosome segregation. Mechanistically, the homeobox (HOX) domain of ONECUT3, serving as the DNA binding domain, occupied the unique genomic regions of INCENP and CDCA8 and transcriptionally activated these 2 genes. We identified a lead compound, C5484617, that functionally targeted the HOX domain of ONECUT3, inhibiting its transcriptional activity on downstream genes, and synergistically resensitized MDS cells to hypomethylating agents. This study revealed that ONECUT3 promoted chromosomal instability by transcriptional activation of INCENP and CDCA8, suggesting potential prognostic and therapeutic roles for targeting high-risk MDS patients with a CK.
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  • 文章类型: Journal Article
    核苷酸结合位点和富含亮氨酸的重复蛋白(NLR)充当关键的细胞内免疫受体。先前的研究报道了拟南芥抗性基因L3(AT1G15890),编码卷曲螺旋(CC)NLR,可导致细菌细胞死亡;然而,其在植物中的功能尚不清楚。本研究描述了本氏烟草L3的全面结构功能分析。瞬时测定的结果显示L3CC结构域足以诱导细胞死亡。前140个氨基酸区段构成可能导致细胞死亡的最小功能区域。YFP标记的L3CC结构域位于质膜,这被认为对L3CC域的功能和自我相互作用至关重要。点突变分析结果表明,L3CC结构域功能受某些特定残基突变的影响,CC结构域中的功能缺失突变影响全长L3的功能。这些研究结果为了解L3的激活机制提供了大量证据。
    Nucleotide-binding sites and leucine-rich repeat proteins (NLRs) act as critical intracellular immune receptors. Previous studies reported an Arabidopsis-resistant gene L3 (AT1G15890), which encoded a coiled-coil (CC) NLR that conferred cell death in bacteria; however, its function in planta remains unclear. This study describes a comprehensive structure-function analysis of L3 in Nicotiana benthamiana. The results of the transient assay showed that the L3 CC domain is sufficient for cell-death induction. The first 140 amino acid segment constituted the minimal function region that could cause cell death. The YFP-labeled L3 CC domain was localized to the plasma membrane, which was considered crucial for the function and self-interaction of the L3 CC domain. The results of point mutations analysis showed that L3 CC domain function is affected by mutations in some specific residues, and loss-of-function mutations in the CC domain affected the function of full-length L3. These study results offered considerable evidence to understand the activation mechanism of L3.
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  • 文章类型: Journal Article
    2-硝基苯胺(2-NA)是一种环境污染物,已被广泛用作有机合成的中间体。环境中2-NA的存在不仅对水生生物有害,而且对人类诱变。在这项研究中,我们构建了表达旧黄酶基因的转基因水稻,ScOYE3,来自酿酒酵母。全面研究了ScOYE3转基因植物对2-NA处理的生化反应及其2-NA植物修复能力。我们的结果表明,水稻幼苗暴露于2-NA胁迫,显示生长抑制和生物量减少。然而,与野生型植物相比,转基因植物表现出对2-NA胁迫的强耐受性。异位表达ScOYE3可以有效保护转基因植株免受2-NA损伤,与野生型植物相比,转基因植物中的活性氧积累更少。我们的植物修复试验表明,转基因植物比野生型植物可以从培养基中消除更多的2-NA。此外,为了更深入地了解ScOYE3介导的水稻2-NA转化机制,进行了组学分析.总之,首次对ScOYE3在2-NA解毒过程中的功能进行了表征,这为老黄酶基因对2-NA的植物修复潜力提供了强有力的理论支持。
    2-nitroaniline (2-NA) is an environmental pollutant and has been extensively used as intermediates in organic synthesis. The presence of 2-NA in the environment is not only harmful for aquatic life but also mutagenic for human beings. In this study, we constructed transgenic rice expressing an Old Yellow Enzyme gene, ScOYE3, from Saccharomyces cerevisiae. The ScOYE3 transgenic plants were comprehensively investigated for their biochemical responses to 2-NA treatment and their 2-NA phytoremediation capabilities. Our results showed that the rice seedlings exposed to 2-NA stress, showed growth inhibition and biomass reduction. However, the transgenic plants exhibited strong tolerance to 2-NA stress compared to wild-type plants. Ectopic expression of ScOYE3 could effectively protect transgenic plants against 2-NA damage, which resulted in less reactive oxygen species accumulation in transgenic plants than that in wild-type plants. Our phytoremediation assay revealed that transgenic plants could eliminate more 2-NA from the medium than wild-type plants. Moreover, omics analysis was performed in order to get a deeper insight into the mechanism of ScOYE3-mediated 2-NA transformation in rice. Altogether, the function of ScOYE3 during 2-NA detoxification was characterized for the first time, which serves as strong theoretical support for the phytoremediation potential of 2-NA by Old Yellow Enzyme genes.
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  • 文章类型: Journal Article
    本研究旨在探讨具有ITIM和Ig结构域的T细胞免疫受体(TIGIT)在肺腺癌(LUAD)中的表达。通过蛋白质印迹测量TIGIT表达,逆转录定量聚合酶链反应。从I-IV期LUAD患者中收集了72个配对的手术标本。用免疫组化法测定手术标本中TIGIT的表达。TIGIT在LUAD组织中过表达。此外,过度表达的TIGIT与晚期临床分期显着相关,淋巴结转移,远处转移,LUAD中TP53突变。此外,TIGIT的高表达与CD4+T细胞纯度呈负相关。TIGIT+CD4+T细胞的高比例预测LUAD患者的总体生存率较差。此外,TIGIT+CD4+T细胞的高比例与CD4+T细胞耗竭密切相关。一起来看,TIGIT在LUAD患者中过度表达。高水平的TIGIT诱导基于CD4+T细胞的免疫调节的改变并预测LUAD患者的不良预后。因此,TIGIT可能是LUAD的潜在生物标志物。
    This study aimed to investigate the T cell immunoreceptor with ITIM and Ig domains (TIGIT) expression in lung adenocarcinoma (LUAD). TIGIT expression was measured by western blot, reverse transcription quantitative polymerase chain reaction. Seventy-two paired surgical specimens were collected from patients with stage I-IV LUAD. The expression of TIGIT in surgical specimens was determined using immunohistochemistry. TIGIT was overexpressed in LUAD tissues. Moreover, overexpressed TIGIT was significantly associated with advanced clinical staging, lymph node metastasis, distant metastasis, and TP53 mutations in LUAD. Moreover, high expression of TIGIT was negatively correlated with purity of CD4+ T cells. High rations of TIGIT+CD4+ T cells predicted poor overall survival of LUAD patients. Additionally, high ratios of TIGIT+CD4+ T cells is closely related to CD4+ T cell depletion. Taken together, TIGIT was overexpressed in LUAD patients. High levels of TIGIT induced the alteration of CD4+ T cell based immunomodulation and predicted poor prognosis of LUAD patients. Therefore, TIGIT can be potential biomarker for LUAD.
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  • 文章类型: Journal Article
    响应Cd胁迫的Cd耐性蛋白SaCTP3,在Sedumalfredii中发现;然而,如何利用CTP基因提高Cd污染土壤的植物修复效率尚不清楚。在这项研究中,确定了景天SaCTP3的植物修复潜力。在过表达SaCTP3的酵母Cd敏感菌株Δycf1中,Cd的积累高于过表达空载体的Δycf1菌株。进一步构建过表达SaCTP3的转基因高粱植株以验证SaCTP3的功效。与野生型植物相比,在500μMCd条件下,过表达SaCTP3的品系表现出更高的Cd积累。SaCTP3过表达植物中的平均Cd含量比WT植物高四倍以上。这伴随着清除ROS的能力增强,过氧化物酶活性显著增加,过氧化氢酶,和超氧化物歧化酶对Cd胁迫的响应。盆栽实验进一步表明,SaCTP3过表达可提高土壤Cd清除能力和光合能力。经过20天的生长,过表达SaCTP3的高粱种植土壤中Cd的平均含量下降了19.4%,而种植野生型植物的土壤中残留的Cd含量仅降低了5.4%。本研究阐明了S.alfredii的SaCTP3的作用,强调其在转基因高粱中的潜在用途,以有效修复Cd。
    The Cd tolerance protein SaCTP3, which responds to Cd stress, was identified in Sedum alfredii; however, how to improve the efficiency of phytoremediation of Cd-contaminated soil using the CTP gene remains unknown. In this study, the phytoremediation potential of SaCTP3 of Sedum alfredii was identified. In the yeast Cd-sensitive strain Δycf1 overexpressing SaCTP3, the accumulation of Cd was higher than that in the Δycf1 strain overexpressing an empty vector. Transgenic sorghum plants overexpression SaCTP3 were further constructed to verify the function of SaCTP3. Compared to wild-type plants, the SaCTP3-overexpressing lines exhibited higher Cd accumulation under 500 μM Cd conditions. The average Cd content inSaCTP3-overexpressing plants is more than four times higher than that of WT plants. This was accompanied by an enhanced ability to scavenge ROS, as evidenced by the significantly increased activities of peroxidase, catalase, and superoxide dismutase in response to Cd stress. Pot experiments further demonstrated that SaCTP3 overexpression resulted in improved soil Cd scavenging and photosynthetic abilities. After 20 days of growth, the average Cd content in the soil planted with SaCTP3-overexpressing sorghum decreased by 19.4%, while the residual Cd content in the soil planted with wild-type plants was only reduced by 5.4%. This study elucidated the role of SaCTP3 from S.alfredii, highlighting its potential utility in genetically modifying sorghum for the effective phytoremediation of Cd.
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