‘圣诞快乐’朱顶红花芽分化研究

采用解剖观测和石蜡切片技术,对朱顶红品种‘圣诞快乐’花芽生长情况、花器官分化和性细胞分化过程进行了研究,以明确朱顶红花芽分化特征,为其花发育、花期调控、杂交育种和系统分类研究提供理论依据。结果表明：‘圣诞快乐’朱顶红每年产生2个花序芽,在第2年完成其内花芽花器官分化,经过低温作用后于第3年盛开,其中第2个花序偶有败育发生;花器官分化过程包括花原基分化期、外花被原基分化期、内花被原基分化期、雄蕊原基分化期、心皮原基分化期,对应的花芽大小分别约为0.02、0.05、0.1、0.2、0.3 cm,所有花器官均为螺旋状向心式发生;朱顶红花药4室,花药壁从外至内由表皮、药室内壁、中层和绒毡层组成,绒毡层类型为分泌型,小孢子减数分裂类型为连续型,四分体排列方式为十字交叉型,成熟花粉粒为2-细胞型;朱顶红雌蕊3心皮,下位子房,中轴胎座,3心室,每室两列倒生胚珠,胚珠为双珠被,厚珠心,具葱型胚囊。     

灰葡萄孢菌AUR1基因真核表达载体的构建、表达及酶活性分析

为了研究灰葡萄孢菌肌糖磷脂酰神经酰胺合成酶(BcAUR1基因)的表达及酶活性,采用RT-PCR方法,利用含有FLAG标签以及BamH Ⅰ、Xho Ⅰ酶切位点的AUR1特异引物从灰葡萄孢菌中扩增得到BcAUR1基因.将BcA UR1基因与穿梭质粒pYES2重组,得到pYES2-BcAUR1质粒采用醋酸锂转化法导入酿酒酵母尿嘧啶突变菌株△yor1中,Western blotting检测肌糖磷脂酰神经酰胺(IPC)合成酶表达,HPLC检测IPC合成酶活力.结果显示pYE S2-BcA UR1在酿酒酵母尿嘧啶突变菌株△yorl中获得表达,pYES2-BcA UR1转化子IPC合成酶活性显著增高,比空载转化子约提高1倍.低浓度的AbA能够抑制空载pYES2酵母转化子生长,但pYES2-BcA UR1酵母转化子能抵抗AbA对菌体生长的抑制.     

Prognostic Value and Clinicopathology Significance of MicroRNA-200c Expression in Cancer: A Meta-Analysis

MiR-200c has been shown to be related to cancer formation and progression. However, the prognostic and clinicopathologic significance of miR-200c expression in cancer remain inconclusive. We carried out this systematic review and meta-analysis to investigate the prognostic value of miR-200c expression in cancer. Pooled hazard ratios (HRs) of miR-200c for overall survival (OS) and progression-free survival (PFS) were calculated to measure the effective value of miR-200c expression on prognosis. The association between miR-200c expression and clinical significance was measured by odds ratios (ORs). Twenty-three studies were included in our meta-analysis. We found that miR-200c was not significantly correlated with OS (HR = 1.41, 95%Cl: 0.95-2.10; P = 0.09) and PFS (HR = 1.12, 95%Cl: 0.68-1.84; P = 0.67) in cancer. In our subgroup analysis, higher expression of miR-200c was significantly associated with poor OS in blood (HR = 2.10, 95%CI: 1.52-2.90, P<0.00001). Moreover, in clinicopathology analysis, miR-200c expression in blood was significantly associated with TNM stage, lymph node metastasis and distant metastasis. MiR-200c may have the potential to become a new blood biomarker to monitor cancer prognosis and progression.     

Nur77 promotes cerebral ischemia–reperfusion injury via activating INF2-mediated mitochondrial fragmentation

Mitochondrial fragmentation drastically regulates mitochondrial homeostasis in brain illness. However, the role of mitochondrial fragmentation in cerebral ischemia–reperfusion (IR) injury remains unclear. Nur77, a regulator of mitochondrial homeostasis, is associated with heart and liver IR injury, but its effects on mitochondrial function in cerebral IR injury has not been studied intensively. The aim of our study is to explore whether cerebral IR injury is modulated by Nur77 via modification of mitochondrial homeostasis. Our results indicated that Nur77 was upregulated in reperfused brain tissues. Genetic ablation of Nur77 reduced infarction area and promoted neuron survival under IR burden. Biochemical analysis demonstrated that Nur77 deletion protected mitochondrial function, attenuated mitochondrial oxidative stress, preserved mitochondrial potential, and blocked mitochondria-related cell apoptosis. In addition, we illustrated that Nur77 mediated mitochondrial damage via evoking mitochondrial fragmentation that occurred through increased mitochondrial fission and decreased fusion. Besides, our results also demonstrated that Nur77 controlled mitochondrial fragmentation via upregulating INF2 in a manner dependent on the Wnt/β-catenin pathway; inhibition of the Wnt pathway abrogated the protective effect of Nur77 deletion on reperfused-mediated neurons. Altogether, our study highlights that the pathogenesis of cerebral IR injury is associated with Nur77 activation followed by augmented mitochondrial fragmentation via an abnormal Wnt/β-catenin/INF2 pathway. Accordingly, Nur77-dependent mitochondrial fragmentation and the Wnt/β-catenin/INF2 axis may represent novel therapeutic targets to reduce cerebral IR injury.     

Antiproliferative homoscalarane sesterterpenes from two Madagascan sponges

Dereplication of the antiproliferative ethyl acetate fraction of the Madagascan sponge Carteriospongia sp. led to the detection and isolation of the two known homoscalarane-type sesterterpenes 1 and 2. Investigation of a similar sponge containing closely related compounds afforded the four new antiproliferative homoscalarane sesterterpenes (3 and 5?7). The structures of all isolated compounds were elucidated by spectroscopic methods, including UV, IR and 1D and 2D NMR. Compounds 1, 3 and 5 displayed submicromolar antiproliferative activity against the A2780 ovarian cell line with IC₅₀ values of 0.65, 0.26 and 0.28 μM, respectively, while compounds 6 and 7 showed moderate activity (4.5 and 8.7 μM, respectively). Compounds 3 and 5 also displayed anti-proliferative activity against the H522-T1 non-small cell lung and A2058 human melanoma cancer cell lines.     

Tn<Emphasis Type="Italic">5</Emphasis> transposase-assisted high-efficiency transformation of filamentous fungus <Emphasis Type="Italic">Phoma herbarum</Emphasis> YS4108

Conventionally, filamentous fungi are transformed by using conidia or protoplasts as recipients. However, induction of sporulation is difficult in some fungi, and protoplasting is an awing, frequently frustrating, and batch-dependent work. In this study, we established a simple and convenient method to prepare single cells from mycelia without enzymatic protoplasting. As a case study on the pathogenic fungus Phoma herbarum YS4108, the single cells could be directly and highly efficiently transformed with the aid of Tn5 transposase. The optimal electric pulse delivery parameters were 25 muF in capacitance, 0.75 kV (0.2-cm cuvette) in voltage, and 400 Omega in resistance, under which the efficiency of transposase-assisted transformation (TNAT) was enhanced to two to threefold compared to that of non-TNAT method, resulting in >230 transformants/cuvette (10(6) recipients). Further cell wall weakening of the single cells by lytic enzymes and linearization of the plasmid were found to have no effects on transformation efficiency, but vector linearization apparently lowered the background growth. The present study for the first time explained that Tn5 transposase could be used to increase transformation efficiency in filamentous fungi, and the method presented here may be of wide applicability in different studies and may be the first choice when transformation efficiency and convenience are priorities and mycelia have to be used as transformation recipients.