DNA demethylase ROS1 prevents inheritable DREB1A/CBF3 repression by transgene-induced promoter methylation in the Arabidopsis ice1-1 mutant

Plant Molecular Biology - In the ros1-defective mutant, DREB1A repression by the transgene-induced promoter methylation of ice1-1 became inheritable across generations even in the absence of the...     

基因枪法获得逆境诱导转录因子DREB1A转基因小麦的研究

以小麦品种H6756和藁城8901作为基因枪转化的靶材料,取其护颖至雌雄蕊原基形成期的幼穗,用含逆境诱导转录因子DREB1A和bar基因的质粒pAHC25轰击胚性愈伤组织,在分别含有5mgL和10mgLBasta溶液的培养基上进行筛选。得到的抗性愈伤组织在不含Basta溶液的培养基上再生培养,获得218棵再生植株。田间涂抹浓度为100mgL的Basta溶液检测后,对抗性植株作PCR检测,获得54棵再生植株。通过对其中20株T1代的PCR和Southern杂交分析,已获得14株含DREB1A和bar基因的转基因小麦植株,其中H675613株,藁城89011株。     

miR-29a/b Enhances Cell Migration and Invasion in Nasopharyngeal Carcinoma Progression by Regulating SPARC and COL3A1 Gene Expression

Nasopharyngeal carcinoma (NPC) is a malignant tumor associated with a genetic predisposition, Epstein-Barr virus infection and chromosomal abnormalities. Recently, several miRNAs have been shown to target specific mRNAs to regulate NPC development and progression. However, the involvement of miRNAs in processes leading to NPC migration and invasion remains to be elucidated. We predicted that miR-29a/b are associated with dysregulated genes controlling NPC through an integrated interaction network of miRNAs and genes. miR-29a/b over-expression in NPC cell lines had no significant effect on proliferation, whereas miR-29b mildly increased the percentage of cells in the G1 phase with a concomitant decrease in the percentage of cells in S phase. Furthermore, we demonstrated that miR-29a/b might be responsible for increasing S18 cell migration and invasion, and only COL3A1 was identified as a direct target of miR-29b despite the fact that both SPARC and COL3A1 were inhibited by miR-29a/b over-expression. Meanwhile, SPARC proteins were increased in metastatic NPC tissue and are involved in NPC progression. Unexpectedly, we identified that miRNA-29b expression was elevated in the serum of NPC patients with a high risk of metastasis. The 5-year actuarial overall survival rates in NPC patients with high serum miR-29b expression was significantly shorter than those with low serum miR-29b expression; therefore, serum miR-29b expression could be a promising prognostic marker.     

RIC-3 Exclusively Enhances the Surface Expression of Human Homomeric 5-Hydroxytryptamine Type 3A (5-HT3A) Receptors Despite Direct Interactions with 5-HT3A, -C, -D, and -E Subunits

Although five 5-hydroxytryptamine type 3 (5-HT3) subunits (A–E) have been cloned, knowledge on the regulation of their assembly is limited. RIC-3 has been identified as a chaperone specific for the pentameric ligand-gated nicotinic acetylcholine and 5-HT₃ receptors. Therefore, we examined the impact of RIC-3 on differently composed 5-HT₃ receptors with the focus on 5-HT3C, -D, and -E subunits. The influence of RIC-3 on these receptor subtypes is supported by the presence of RIC3 mRNA in tissues expressing at least one of the subunits 5-HT3C, -D, and -E. Furthermore, immunocytochemical studies on transfected mammalian cells revealed co-localization in the endoplasmic reticulum and direct interaction of RIC-3 with 5-HT3A, -C, -D, and -E. Functional and pharmacological characterization was performed using HEK293 cells expressing 5-HT3A or 5-HT3A + 5-HT3B (or -C, -D, or -E) in the presence or absence of RIC-3. Ca²⁺ influx analyses revealed that RIC-3 does not influence the 5-HT concentration-response relationship on 5-HT₃A receptors but leads to differential increases of 5-HT-induced maximum response (E_max) on cells expressing different subunits. Increases of E_max were due to analogously enhanced B_max values for binding of the 5-HT₃ receptor antagonist [³H]GR65630. The observed enhanced cell surface expression of the tested 5-HT3 subunit combinations correlated with the increased surface expression of 5-HT3A as determined by flow cytometry. In conclusion, we showed that RIC-3 can interact with 5-HT3A, -C, -D, and -E subunits and predominantly enhances the surface expression of homomeric 5-HT₃A receptors in HEK293 cells. These data implicate a possible role of RIC-3 in determining 5-HT₃ receptor composition in vivo.     

TPK1, a Ca(2+)-regulated Arabidopsis vacuole two-pore K(+) channel is activated by 14-3-3 proteins

The vacuole represents a pivotal plant organelle for management of ion homeostasis, storage of proteins and solutes, as well as deposition of cytotoxic compounds. Ion channels, pumps and carriers in the vacuolar membrane under control of cytosolic factors provide for ionic and metabolic homeostasis between this storage organelle and the cytoplasm. Here we show that AtTPK1 (KCO1), a vacuolar membrane localized K(+) channel of the TPK family, interacts with 14-3-3 proteins (general regulating factors, GRFs). Following in planta expression TPK1 and GRF6 co-localize at the vacuolar membrane. Co-localization of wild-type TPK1, but not the TPK1-S42A mutant, indicates that phosphorylation of the 14-3-3 binding motif of TPK1 represents a prerequisite for interaction. Pull-down assays and surface plasmon resonance measurements revealed GRF6 high-affinity interaction with TPK1. Following expression of TPK1 in yeast and isolation of vacuoles, patch-clamp studies identified TPK1 as a voltage-independent and Ca(2+)-activated K(+) channel. Addition of 14-3-3 proteins strongly increased the TPK1 activity in a dose-dependent manner. However, an inverse effect of GRF6 on the activity of the slow-activating vacuolar (SV) channel was observed in mesophyll vacuoles from Arabidopsis thaliana. Thus, TPK1 seems to provide for a Ca(2+)- and 14-3-3-sensitive mechanism capable of controlling cytoplasmic potassium homeostasis in plants.     

miR-769-3p 对甲型 H1N1流感病毒核蛋白表达的调控

目的:预测靶向甲型流感病毒核蛋白(NP)基的微小 RNA(miRNA),并检测其对 NP 表达的影响.方法:从miRBase 数据库中获取人成熟 miRNA 序列,利用 miRanda 软件预测潜在靶向流感病毒 A/FM/1/47(H1N1) NP 基的人 miRNA;通过双萤光素酶报告基系统及 Western 印迹验证所预测的 miRNA 对 NP 表达的影响.结果:用 miRanda软件在流感病毒 A/FM/1/47(H1N1) NP 基上预测得到分值及最小结合自由能均较好的 miR-769-3p;双萤光素酶报告基结果显示 miR-769-3p 能显著降低报告基载体萤光素酶的表达;Western 印迹结果显示 miR-769-3p 能明显抑制 NP 的表达,但突变 NP 基上的 miR-769-3p 结合位点后,miR-769-3p 不能抑制 NP 的表达.结论:miR-769-3p 可靶向流感病毒 A/FM/1/47(H1N1) NP 基并抑制 NP 的表达,为抗甲型流感病毒的 miRNA 药物研发提供了据和潜在药物靶标.     

Gene NANA regulates cell proliferation in Arabidopsis thaliana shoot apical meristem without interaction with CLV1, CLV2, CLV3

A constancy of stem cell pool in shoot apical meristem of Arabidopsis thaliana is provided by a genetic regulation system with negative feedback loop based on the interaction of the gene WUS, which maintains indeterminate state of cells, with CLV genes, which restrict the level of WUS expression and stem cell pool size. clv mutations lead to an increase in the pool of stem cells in the apical and floral meristems and wus mutation leads to the opposite effect. Mutation na (nana), like wus mutation, causes premature termination of shoot apical meristem function, although it does not affect the activity of the flower meristem. To elucidate the role of NA in the control of shoot apical meristem functioning, the interaction of NA with CLV genes were investigated. Additive phenotype of double mutants na clv1, na clv2-1, and na clv3-2 indicates that the NA gene makes an independent contribution to the functioning of the shoot apical meristem. It is assumed that the NA gene controls apical meristem cell proliferation during the transition to the reproductive phase of plant development, acting much later and independently of the genes WUS-CLV.     

Characterization of GPI2A,a Potent Inhibitor of HIV-1 Gene Expression and Viral Replication

Abstract

Fully thioated antisense molecules are often cytotoxic and non-specitic in action. GPI2A is thioated at 7 base positions. GPI2A posses sequence-specific activity against HIV-1 gene expression and viral replication without sigdcant cytotoxicity. Partial thioation did not compromise its uptake, cellular distribution and nuclease resistance.     

新鞘氨醇杆菌属9-1的纤维素酶基因Nspcel8A的克隆表达与酶学特性

木质纤维素转化成燃料酒精是缓解能源和环境危机的途径之一.降低将木质纤维素转化成生物燃料的生产成本,需要提高纤维素酶产量或筛选到具更高酶活性的纤维素酶.新鞘氨醇杆菌(Genus Novosphin-gobium)属于鞘氨醇杆菌科(Sphingomonads),该科的细菌新陈代谢多样化,能够降解有机化合物,也可应用于木质素的降解,但目前新鞘氨醇杆菌属细菌的纤维素酶基因的研究未见报道.本研究对新鞘氨醇杆菌属细菌菌株9-1的纤维素酶基因Nspcel8A进行了克隆表达和酶学特性鉴定.Nspcel8A含有属于糖基水解酶家族8的催化结构域.该酶在大肠杆菌中实现了异源表达并获得了表达产物.Nspcel8A对羧甲基纤维素(car-boxymethylcellulose,CMC)的最适作用pH值和温度分别为4.0和40℃,Nspcel8A具有良好的pH值稳定性,在pH值3.5～11.0范围内放置24 h后能够保持60％以上的酶活力.Nspcel8A对CMC的Km值为10 mg/mL,Vmax为14 μmol·min-1·mg-1.底物特异性测试显示Nspcel8A对CMC有最高的酶活力(8.40 U/mg),但对不可溶纤维维如磷酸膨胀纤维素和Avicel只有较低的酶活力或没有酶活.高效液相色谱法分析显示Nsp-ce18A 不能降解纤维二糖、纤维三糖、纤维四糖,能把纤维五糖部分降解成纤维二糖和纤维三糖,能把纤维六糖降解为纤维二糖、纤维三糖和纤维四糖,并以纤维三糖为主.以上结果显示Nspcel8A是一个内切葡聚糖酶,由于它不能水解结晶纤维素,说明它不是Novosphingobium sp.9-1主要的纤维素降解酶.