中国梭梭属植物历史分布格局及其驱动机制

梭梭属(Haloxylon)植物是藜科的古老孑遗物种, 探究末次间冰期(last interglacial period, LIG)和末次盛冰期(last glacial maximum period, LGM)以来中国梭梭属植物的历史地理分布格局及其驱动机制, 对了解气候变化背景下旱生植物区系的发展与演化具有重要意义。本研究利用梭梭属85个自然分布点数据(60条梭梭(Haloxylon ammodendron)分布记录、25条白梭梭(H. persicum)分布记录)和2套环境因子数据, 整合GIS空间分析和9种物种分布模型, 分析了梭梭属末次间冰期以来的地理分布格局变化及其驱动机制。基于62个梭梭属种群的叶绿体基因测序数据, 利用最小成本路径方法, 模拟了末次间冰期以来梭梭属可能的扩散路径。利用R软件prcomp函数对影响梭梭属分布的环境变量进行主成分分析(principal component analysis, PCA), 评价了环境变量对梭梭属适宜分布的贡献, 并分析了关键变量与分布适宜性的相关性。结果表明: (1)集成模型的模拟精度较单一模型显著提升, 且对白梭梭的模拟精度高于梭梭; (2)末次间冰期以来, 梭梭属植物的分布均经历了显著收缩和冰后期扩张, 末次间冰期至末次盛冰期时期, 在准噶尔盆地、塔里木盆地西部广泛分布的梭梭大面积向西退缩至避难所(准噶尔盆地西北缘和塔里木盆地西北缘); 白梭梭从准噶尔盆地、塔里木盆地西端向南退缩至避难所(准噶尔盆地南缘); 末次盛冰期至今, 梭梭向东沿甘肃北部扩张直至内蒙古西部阿拉善荒漠, 白梭梭向东北方向小范围扩张, 占据了准噶尔盆地西部和南缘; (3)末次间冰期以来的气候波动对梭梭属植物的分布存在较大限制, 降水因子主导了梭梭属适宜分布面积的变化, 温度因子影响了梭梭属分布适宜性的高低。     

Carbon starvation reduces carbohydrate and anthocyanin accumulation in red-fleshed fruit via trehalose 6-phosphate and MYB27

Kiwifruit (Actinidia spp.) is a recently domesticated fruit crop with several novel-coloured cultivars being developed. Achieving uniform fruit flesh pigmentation in red genotypes is challenging. To investigate the cause of colour variation between fruits, we focused on a red-fleshed Actinidia chinensis var. chinensis genotype. It was hypothesized that carbohydrate supply could be responsible for this variation. Early in fruit development, we imposed high or low (carbon starvation) carbohydrate supplies treatments; carbohydrate import or redistribution was controlled by applying a girdle at the shoot base. Carbon starvation affected fruit development as well as anthocyanin and carbohydrate metabolite concentrations, including the signalling molecule trehalose 6-phosphate. RNA-Seq analysis showed down-regulation of both gene-encoding enzymes in the anthocyanin and carbohydrate biosynthetic pathways. The catalytic trehalose 6-phosphate synthase gene TPS1.1a was down-regulated, whereas putative regulatory TPS7 and TPS11 were strongly up-regulated. Unexpectedly, under carbon starvation MYB10, the anthocyanin pathway regulatory activator was slightly up-regulated, whereas MYB27 was also up-regulated and acts as a repressor. To link these two metabolic pathways, we propose a model where trehalose 6-phosphate and the active repressor MYB27 are involved in sensing the carbon starvation status. This signals the plant to save resources and reduce the production of anthocyanin in fruits.     

Metabotropic Glutamate Receptor 1 Expression and Its Polymorphic Variants Associate with Breast Cancer Phenotypes

Several epidemiological studies have suggested a link between melanoma and breast cancer. Metabotropic glutamate receptor 1 (GRM1), which is involved in many cellular processes including proliferation and differentiation, has been implicated in melanomagenesis, with ectopic expression of GRM1 causing malignant transformation of melanocytes. This study was undertaken to evaluate GRM1 expression and polymorphic variants in GRM1 for associations with breast cancer phenotypes. Three single nucleotide polymorphisms (SNPs) in GRM1 were evaluated for associations with breast cancer clinicopathologic variables. GRM1 expression was evaluated in human normal and cancerous breast tissue and for in vitro response to hormonal manipulation. Genotyping was performed on genomic DNA from over 1,000 breast cancer patients. Rs6923492 and rs362962 genotypes associated with age at diagnosis that was highly dependent upon the breast cancer molecular phenotype. The rs362962 TT genotype also associated with risk of estrogen receptor or progesterone receptor positive breast cancer. In vitro analysis showed increased GRM1 expression in breast cancer cells treated with estrogen or the combination of estrogen and progesterone, but reduced GRM1 expression with tamoxifen treatment. Evaluation of GRM1 expression in human breast tumor specimens demonstrated significant correlations between GRM1 staining with tissue type and molecular features. Furthermore, analysis of gene expression data from primary breast tumors showed that high GRM1 expression correlated with a shorter distant metastasis-free survival as compared to low GRM1 expression in tamoxifen-treated patients. Additionally, induced knockdown of GRM1 in an estrogen receptor positive breast cancer cell line correlated with reduced cell proliferation. Taken together, these findings suggest a functional role for GRM1 in breast cancer.     

Plant rhizosphere influence on microbial C metabolism: the role of elevated CO2, N availability and root stoichiometry

Microbial decomposer C metabolism is considered a factor controlling soil C stability, a key regulator of global climate. The plant rhizosphere is now recognized as a crucial driver of soil C dynamics but specific mechanisms by which it can affect C processing are unclear. Climate change could affect microbial C metabolism via impacts on the plant rhizosphere. Using continuous ¹³C labelling under controlled conditions that allowed us to quantify SOM derived-C in all pools and fluxes, we evaluated the microbial metabolism of soil C in the rhizosphere of a C4 native grass exposed to elevated CO₂ and under variation in N concentrations in soil and in plant root C:N stoichiometry. Our results demonstrated that this plant can influence soil C metabolism and further, that elevated CO₂ conditions can alter this role by increasing microbial C efficiency as indicated by a reduction in soil-derived C respiration per unit of soil C-derived microbial biomass. Moreover, under elevated CO₂ increases in soil N, and notably, root tissue N concentration increased C efficiency, suggesting elevated CO₂ shifted the stoichiometric balance so N availability was a more critical factor regulating efficiency than under ambient conditions. The root C:N stoichiometry effect indicates that plant chemical traits such as root N concentration are able to influence the metabolism of soil C and that elevated CO₂ conditions can modulate this role. Increased efficiency in soil C use was associated with negative rhizosphere priming and we hypothesize that the widely observed phenomenon of rhizosphere priming may result, at least in part, from changes in the metabolic efficiency of microbial populations. Observed changes in the microbial community support that shifting microbial populations were a contributing factor to the observed metabolic responses. Our case study points at greater efficiency of the SOM-degrading populations in a high CO₂, high N world, potentially leading to greater C storage of microbially assimilated C in soil.     

MicroRNA-30c serves as an independent biochemical recurrence predictor and potential tumor suppressor for prostate cancer

MicroRNA-30c (miR-30c) acts as a tumor suppressor or a tumor promoter in various human malignancies. However, the involvement of miR-30c in prostate cancer (PCa) is still unclear. The aim of this study was to investigate the molecular function and the clinical significance of miR-30c in PCa. Expression levels of miR-30c in PCa tissues and cells were detected by quantitative real-time-PCR (qRT-PCR). Additionally, the associations of miR-30c expression with clinicopathological features and prognosis in PCa patients were analyzed. The potential role of miR-30c in tumorigenesis of PCa cells was further evaluated by in vitro cell assays. MiR-30c was significantly down-regulated in PCa tissues and cells compared with the corresponding controls (P < 0.05). In addition, the downregulation of miR-30c in PCa tissues was significantly associated with higher Gleason score (P = 0.009), advanced pathological stage (P = 0.016) and biochemical recurrence (P = 0.034). Moreover, Kaplan–Meier survival analysis showed that the reduced expression of miR-30c was correlated with shorter biochemical recurrence-free survival (P = 0.023). The multivariate analysis also identified miR-30c as an independent prognostic predictor for biochemical recurrence-free survival in patients with PCa. Furthermore, the enforced expression of miR-30c suppressed proliferation, migration and invasion of PCa cells in vitro. Our data indicated the involvement of miR-30c in PCa progression and suggested its potential role as an independent predictor of biochemical recurrence in PCa. On cellular level, miR-30c may function as a tumor suppressor for PCa cells by inhibiting tumor cell proliferation, migration and invasion.     

Disentangling root responses to climate change in a semiarid grassland

Future ecosystem properties of grasslands will be driven largely by belowground biomass responses to climate change, which are challenging to understand due to experimental and technical constraints. We used a multi-faceted approach to explore single and combined impacts of elevated CO₂ and warming on root carbon (C) and nitrogen (N) dynamics in a temperate, semiarid, native grassland at the Prairie Heating and CO₂ Enrichment experiment. To investigate the indirect, moisture mediated effects of elevated CO₂, we included an irrigation treatment. We assessed root standing mass, morphology, residence time and seasonal appearance/disappearance of community-aggregated roots, as well as mass and N losses during decomposition of two dominant grass species (a C₃ and a C₄). In contrast to what is common in mesic grasslands, greater root standing mass under elevated CO₂ resulted from increased production, unmatched by disappearance. Elevated CO₂ plus warming produced roots that were longer, thinner and had greater surface area, which, together with greater standing biomass, could potentially alter root function and dynamics. Decomposition increased under environmental conditions generated by elevated CO₂, but not those generated by warming, likely due to soil desiccation with warming. Elevated CO₂, particularly under warming, slowed N release from C₄—but not C₃—roots, and consequently could indirectly affect N availability through treatment effects on species composition. Elevated CO₂ and warming effects on root morphology and decomposition could offset increased C inputs from greater root biomass, thereby limiting future net C accrual in this semiarid grassland.     

TAT-凋亡素融合蛋白的表达及其抗肿瘤活性

凋亡素(apoptin)由鸡贫血病毒vp3基因编码,能特异地诱导肿瘤细胞凋亡而对正常细胞 没有毒性,为了获得可转导入细胞内部的凋亡素,将人工合成的编码TAT蛋白转导结构域的DNA片段与凋亡素编码基因克隆入质粒pET-28a内,构建出表达融合蛋白TAT-apoptin的原核表达载体pET-28a-TAT-apoptin.在大肠杆菌Rosetta（DE3）中表达融合蛋白,利用IDA -Ni2+ 亲和柱纯化,葡聚糖凝胶G 25除去尿素后得到可溶的变性蛋白.纯化后的TAT apoptin加入体外培养的人脐静脉内皮细胞(HUVECs)和人肺癌Anip973细胞,对照组加入TAT-麦芽糖结合蛋白（TAT-MBP）. 经免疫组化检测,转导1 h后TAT-MBP分布于以上两种细胞的胞浆和胞核,TAT-apoptin则主要分布于2种细胞的胞浆内,转导24 h后TAT-MBP的亚细胞定位没有变化,TAT-apoptin分别定位于HUVECs的胞浆和Anip973的胞核中.脱氧核糖核苷酸末端转移酶介导的缺口末端标记法（TUNEL）显示转导48 h后,TAT-MBP处理过的 HUVECs和Anip973细胞、TAT-apoptin处理过的HUVECs没有明显改变,而TAT-apoptin处理过的Anip973细胞大量凋亡.以上结果表明TAT apoptin融合蛋白在肿瘤治疗上有潜在的应用价值.     

β连环素在新生儿细支气管的表达与研究

目的研究β-cat在新生儿细支气管中的表达情况,探讨β-cat在新生儿支气管发育中的作用。方法采用免疫组化(SP)法,检测22例尸检新生儿β-cat、GSK-3β在细支气管上皮细胞的表达,以12例儿童为对照。结果β-cat在新生儿组有6例出现细胞膜表达降低、3例出现胞质表达、2例胞核表达;对照组中2例胞膜表达减少,1例胞质表达。β-cat的平均光密度值在新生儿组为0·112±0·024,对照组为0·128±0·037。两组比较P>0·05,无显著性差异;GSK-3β平均光密度值在对照组为0·147±0·037,新生儿组为0·115±0·028,两组比较P<0·05,有显著性差异。结论β-cat在新生儿细支气管的异位表达,提示Wnt信号与支气管的发育成熟有关。     

Targeting CD24 for treatment of ovarian cancer by short hairpin RNA

Background aimsCD24 is markedly overexpressed in ovarian cancer and plays a critical role in ovarian cancer survival and metastasis, rendering it an interesting target for anti-tumor therapy. Using short hairpin RNA (shRNA) targeting CD24, we aimed to investigate the anti-tumor efficacy of CD24 knockdown in ovarian cancer cells in vitro and in vivo.MethodsCD24 shRNA vector (CD24–shRNA) and empty plasmid vector (EP) were transfected into ovarian cancer SKOV3 cells and the knockdown efficacy assessed by Western blot analysis. The effects of CD24 knockdown in SKOV3 cells in vitro, including cell viability and apoptosis, were determined using methyl thiazolyl blue tetrazolium bromide (MTT), flow cytometry and propidium iodide (PI) staining assays. The effects in vivo of CD24 knockdown on angiogenesis, cell proliferation and apoptosis were assessed using immunohistochemistry against CD31, proliferating cell nuclear antigen (PCNA) and terminal deoxynucleotidyl transferase-mediated nick end-labeling (TUNEL) assays.ResultsTransfection of CD24–shRNA effectively down-regulated CD24 expression in vitro and in vivo. Administration of CD24–shRNA into nude mice bearing ovarian cancer significantly suppressed tumor volume growth.ConclusionsKnockdown of CD24 expression by CD24–shRNA significantly inhibited cell viability and induced apoptosis of SKOV3 cells in vitro. Administration with CD24–shRNA in vivo suppressed tumor volume increase by microvessel density (MVD) decrease, cell proliferation inhibition and apoptosis induction. All the data suggested that knockdown of CD24 by shRNA might be a potential therapeutic approach against human ovarian cancer.