施钾对苜蓿上牛角花齿蓟马产卵选择、生长发育、 成虫寿命和繁殖力的影响

【目的】为了探讨施钾对苜蓿上牛角花齿蓟马Odontothrips loti的产卵选择、生长发育、成虫寿命和繁殖力的影响,明确施钾苜蓿叶片营养物含量与牛角花齿蓟马生命参数的关系。【方法】在不同钾量(40, 60, 80和100 mg/kg)处理下(以不施钾作为对照),观察记录牛角花齿蓟马在紫花苜蓿品种甘农3号Medicago sativa cv. Gannong No. 3叶片上的产卵量,幼期各龄期发育历期和存活率以及二代成虫的寿命和繁殖力,同时测定不同施钾量下苜蓿叶片的可溶性糖、游离氨基酸及钾含量。【结果】随着施钾量的增加,牛角花齿蓟马在苜蓿叶片上的产卵量(粒/复叶)先降低后升高,在60 mg/kg钾处理降幅最大,较对照降低了45.58%;卵孵化率和1-2龄若虫的存活率变化不显著,但3-4龄若虫的存活率和幼期总存活率显著下降,分别在100 mg/kg 和80 mg/kg钾处理下降幅最大,较对照分别下降了54.36%和48.48%。不同施钾量下苜蓿叶片上牛角花齿蓟马卵和1-2龄若虫发育历期无显著变化,3-4龄若虫及幼期总发育历期均延长;牛角花齿蓟马二代成虫的繁殖力均显著下降,成虫寿命显著缩短(40 mg/kg钾处理除外)。施钾后,苜蓿叶片可溶性糖含量、钾含量和糖氮比增大,游离氨基酸含量减少。相关关系分析表明,苜蓿叶片钾含量与牛角花齿蓟马幼期总存活率和成虫繁殖力无显著相关性,而苜蓿叶片可溶性糖含量和糖氮比均与3-4龄若虫存活率和繁殖力极显著负相关,与幼期总存活率呈显著负相关。【结论】施钾苜蓿对牛角花齿蓟马成虫产卵产生显著的排趋性;施钾提高了苜蓿叶片的可溶性糖含量及糖氮比,不利于若虫的生长发育,并使成虫寿命缩短、繁殖力下降,对牛角花齿蓟马产生了显著的抗生作用。     

PML Suppresses Influenza Virus Replication by Promoting FBXW7 Expression

Virologica Sinica - Influenza A viruses (IAV) are responsible for seasonal flu epidemics, which can lead to high morbidity and mortality each year. Like other viruses, influenza virus can hijack...     

敲低去泛素化酶USP13抑制K562细胞的增殖*

目的:研究去泛素化酶USP13对人慢性髓系白血病细胞系K562增殖和凋亡的影响,并进行初步的机制探究。方法:构建pLKO.1-shUSP13-GFP慢病毒干涉载体,慢病毒包装后感染并建立稳定敲低USP13的K562细胞株。免疫印迹检测K562细胞中USP13蛋白的敲低效率。流式细胞术分析敲低USP13对K562细胞增殖和凋亡的影响。免疫共沉淀和蛋白质泛素化实验探究USP13调控K562细胞的分子机制。结果:成功构建pLKO.1-shUSP13-GFP慢病毒干涉载体,同时利用慢病毒体系获得稳定敲低USP13的K562细胞株。流式细胞术结果显示,敲低USP13促进K562细胞凋亡、抑制细胞增殖。分子机制研究发现,敲低USP13通过增强c-Myc泛素化进而导致其蛋白质水平降低。结论:初步揭示了USP13调控K562细胞增殖和凋亡的分子机制,为治疗慢性髓系白血病提供了潜在的靶点。     

MA诱导方案与DA诱导方案对老年急性髓系白血病患者血清炎症因子及复发率的影响

目的:探讨米托蒽醌联合阿糖胞苷(MA方案)与柔红霉素联合阿糖胞苷(DA方案)对老年急性髓系白血病(AML)患者血清炎症因子及复发率的影响。方法:选取2015年1月~2018年1月期间深圳市人民医院收治的老年AML患者129例,根据治疗方案的不同将患者分为DA组(n=64,DA方案治疗)和MA组(n=65,MA方案治疗),比较两组患者疗效、炎症因子、不良反应及复发情况。结果:MA组治疗后的临床总有效率高于DA组(P<0.05)。两组患者治疗后血清干扰素γ诱导蛋白-10(IP-10)、巨噬细胞炎症蛋白-1α(MIP-1α)及可溶性细胞间黏附分子1(sICAM-1)水平均降低,且MA组低于DA组(P<0.05)。MA组完全缓解患者中累计复发率低于DA组(P<0.05)。两组不良反应发生率比较无差异(P>0.05)。结论:与DA诱导方案相比,MA诱导方案治疗老年AML患者,可有效改善炎症因子水平,减少复发,且用药安全性较好。     

转录因子PU.1的最新研究进展

PU.1是ETS转录因子家族(E26 transformation-specific family)的成员,在机体多种组织发育中发挥重要作用。近年来的研究发现,PU.1不仅在造血谱系的确定和分化中起作用,而且还在机体免疫、脂肪形成、组织纤维化、神经发育中发挥功能。在造血及免疫等系统中,PU.1与多个靶基因形成复杂的调节网络,并且PU.1受组蛋白修饰和非编码RNA等表观遗传的调控,参与细胞增殖、分化等多个过程,对维持细胞稳态具有一定意义。PU.1与红细胞白血病、前B细胞急性淋巴细胞白血病、急性髓细胞白血病、过敏性疾病、类风湿性关节炎、肥胖相关疾病、骨硬病、神经胶质瘤等疾病的发生相关。该文从功能方面阐述PU.1的最新研究进展,为该基因和ETS家族的后续研究提供新思路。     

Construction of a robust prognostic model for adult adrenocortical carcinoma: Results from bioinformatics and real-world data

This study aims to construct a robust prognostic model for adult adrenocortical carcinoma (ACC) by large-scale multiomics analysis and real-world data. The RPPA data, gene expression profiles and clinical information of adult ACC patients were obtained from The Cancer Proteome Atlas (TCPA), Gene Expression Omnibus (GEO) and The Cancer Genome Atlas (TCGA). Integrated prognosis-related proteins (IPRPs) model was constructed. Immunohistochemistry was used to validate the prognostic value of the IPRPs model in Fudan University Shanghai Cancer Center (FUSCC) cohort. 76 ACC cases from TCGA and 22 ACC cases from GSE10927 in NCBI’s GEO database with full data for clinical information and gene expression were utilized to validate the effectiveness of the IPRPs model. Higher FASN (P = .039), FIBRONECTIN (P < .001), TFRC (P < .001), TSC1 (P < .001) expression indicated significantly worse overall survival for adult ACC patients. Risk assessment suggested significantly a strong predictive capacity of IPRPs model for poor overall survival (P < .05). IPRPs model showed a little stronger ability for predicting prognosis than Ki-67 protein in FUSCC cohort (P = .003, HR = 3.947; P = .005, HR = 3.787). In external validation of IPRPs model using gene expression data, IPRPs model showed strong ability for predicting prognosis in TCGA cohort (P = .005, HR = 3.061) and it exhibited best ability for predicting prognosis in GSE10927 cohort (P = .0898, HR = 2.318). This research constructed IPRPs model for predicting adult ACC patients’ prognosis using proteomic data, gene expression data and real-world data and this prognostic model showed stronger predictive value than other biomarkers (Ki-67, Beta-catenin, etc) in multi-cohorts.     

Distribution of the cytoskeletal protein,Nestin, in acute leukemia

Abstract

Nestin is a neuroepithelial stem cell marker that is expressed in some types of tumor cells. Recent reports suggest that Nestin may be closely related to malignant cell proliferation and migration. Acute leukemia (AL) is characterized by a lack of differentiation, which results in uncontrolled proliferation in the bone marrow and accumulation of immature cells. The expression and function of Nestin in AL is unclear. We investigated Nestin immunohistochemical patterns of 87 patients that included 47 cases of acute myeloid leukemia (AML) and 40 cases of acute lymphoblastic leukemia (ALL), and 20 patients in complete remission (CR) from AML or ALL. We also investigated the clinico-pathological features of 87 cases of AL and their CR and overall survival (OS). Nestin was expressed in leukemic blasts and mature granulocytic cells in most cases (39/47) of AML. Conversely, Nestin was expressed in mature granulocytic cells in fewer cases (6/40) of ALL, but not in blasts. Nestin expression appeared in leukemic blasts of AML, but not ALL. Nestin expression in AML blast cells was not associated with CR or OS. We provide evidence that Nestin is expressed in AL and might be a useful immunohistochemical marker for identifying AML and ALL.     

Modifcation of the French Azure C Tissue Stain

A staining procedure for monocytes in specimens of blood and bone marrow was developed. The technique was a two step procedure in which unfixed cells were exposed first to a methanolic solution of C.I. basic blue 54. Next, an aqueous alkaline buffered solution of C.I. basic blue 141 was added to the first staining solution. After staining for 10 min in the solution with two stains, slides or coverslips were washed for 5 sec in pH 5.6 phosphate buffer and drained dry. The cytoplasm of monocytes stained intensely deep purple and frequently nuclei were stained red. Similar staining was not found in other types of normal or abnormal blood and bone marrow cells.