小鼠初级听皮质神经元的强度调谐特性与机制分析

强度是声音的基本参数之一,听神经元的强度调谐在听觉信息处理方面具有重要意义．以往研究发现γ-氨基丁酸(γ-aminobutyric acid, GABA)能抑制性输入在强度调谐的形成过程中起重要作用,但对抑制性输入与局部神经回路之间的关系并不清楚．本实验通过在体细胞外电生理记录和神经药理学方法,分析了小鼠初级听皮质神经元的强度调谐特性,结果显示：单调型神经元在声刺激强度自中等强度增高时潜伏期缩短(P < 0.05)且发放持续时间延长(P < 0.05),非单调型神经元在声刺激强度自最佳强度增高时潜伏期不变且发放持续时间缩短(P < 0.01)．注射GABA能阻断剂荷包牡丹碱(bicuculline, Bic)后,39.3%的神经元强度调谐类型不变,42.9%的神经元非单调性减弱,17.9%的神经元非单调性增强．表明GABA能抑制并非是形成非单调性的唯一因素,兴奋性输入本身的非单调性和高阈值非GABA能抑制的激活也可能在其中发挥作用．推测由兴奋性和抑制性输入所构成的局部神经功能回路及其整合决定了听皮质神经元的强度调谐特性．     

苦瓜叶片结构与白粉病抗性的关系

以不同抗白粉病的苦瓜品系幼苗为材料,对它们的叶片及上下表皮厚度、栅栏组织及海绵组织厚度、叶片结构紧密度及疏松度、蜡质含量、比叶重、气孔及茸毛密度等叶片结构进行观察比较,探讨苦瓜白粉病抗性与其主要叶片结构指标的关系。结果显示:（1）抗病苦瓜品系叶片的蜡质含量显著高于感病品系,与病情指数呈显著负相关关系,蜡质层是其抵抗和延迟病原菌侵入的一个有力结构屏障。（2）感病品系叶片的气孔和叶背面茸毛数量显著多于抗病品系,且叶背面的气孔及茸毛密度与病情指数呈显著正相关关系,即气孔和茸毛越少越抗病。（3）抗病苦瓜品系的叶片栅栏组织以及海绵组织排列整齐、紧密,而高感品系的叶片组织出现大量孔隙,较难观察到完整细胞。（4）抗病品系叶片厚度、下表皮厚度、栅栏组织厚度、叶片结构紧密度明显高于感病品系,而感病品系的海绵组织厚度、叶片结构疏松度明显高于抗病品系;且苦瓜比叶重与其白粉病抗性关系不大。研究认为,苦瓜叶片蜡质含量、叶背面气孔及茸毛密度可以作为苦瓜白粉病抗性鉴定的参考指标。     

自发性高血压大鼠和Wistar大鼠脑动脉平滑肌细胞膜电流的比较

目的:探讨自发性高血压大鼠(SHR)和Wistar大鼠脑动脉(BA)平滑肌细胞膜电流的异同。方法:应用全细胞膜片钳技术研究SHR和Wistar大鼠BA平滑肌细胞在电流密度、电流组成以及自发性瞬时外向K+电流(STOCs)特性的异同。结果:①当指令电压为0、+20、+40和+60mV时,SHR与Wistar大鼠BA平滑肌细胞间电流密度存在统计学差异(P<0.01)。②SHR与Wistar大鼠BA平滑肌细胞膜电流都对1 mmol/L电压依赖的K+通道(Kv)阻断剂4AP和1 mmol/L大电导Ca2+激活K+通道(BKCa)阻断剂TEA敏感。③SHR的STOCs发放频率和电流幅度都远大于Wistar大鼠。1 mmol/LTEA基本完全阻断STOCs通道电流,而4-AP对STOCs没有影响。结论:SHR和Wistar大鼠脑动脉平滑肌细胞的电流密度存在差异,两种平滑肌细胞外向电流都由BKCa和Kv通道组成。SHR大鼠平滑肌细胞更易诱发由BKCa通道介导的STOCs。     

鸭甲肝病毒3型2012年山东分离株VP1基因的序列分析

为揭示近年来鸭甲肝病毒3型(DHAV-3)中国分离株VP1基因的遗传变异规律,本研究对2012年从山东省分离到的13株DHAV-3的VP1基因分别进行PCR扩增、序列测序与分析。结果显示,13株DHAV-3的VP1基因均由720个核苷酸组成,共编码240个氨基酸,核苷酸序列和氨基酸序列同源性分别为94.6%～99.9%和95.0%～100%。与GenBank中公布的31株DHAV-3的VP1基因的核苷酸和氨基酸序列同源性分别为92.5%～100%和90.8%～100%。系统进化分析显示,DHAV-3可分为两个基因型,其中除疫苗毒B63之外所有中国分离株均属于GⅠ型,越南分离毒株主要属于GⅡ型S1亚型,而韩国分离株组成GⅡ型中的S2亚型,具有明显的地域特征。     

Targeted delivery of a phosphopeptide prodrug inhibits the proliferation of a human glioma cell line

Peptides are ideal candidates for developing therapeutics. Polo-like kinase 1 is an important regulatory protein in the cell cycle and contains a C-terminal polo-box domain, which is the hallmark of this protein family. We developed a peptide inhibitor of polo-like kinase 1 that targets its polo-box domain. This new phosphopeptide, cRGDyK-S-S-CPLHSpT, preferentially penetrates the cancer cell membrane mediated by the integrin receptor, which is expressed at high levels by cancer cells. In the present study, using high performance liquid chromatography and mass spectroscopy, we determined the stability of cRGDyK-S-S-CPLHSpT and its cleavage by glutathione under typical conditions for cell culture. We further assessed the ability of the peptide to inhibit the proliferation of the U87MG glioma cell line. The phosphorylated peptide was stable, and the disulfide bond of cRGDyK-S-S-CPLHSpT was cleaved in 50 mM glutathione. This peptide inhibited the growth of cancer cells and changed their morphology. Therefore, we conclude that the phosphopeptide shows promise as a prodrug and has a high potential to act as an anticancer agent by inhibiting polo-like kinase 1 by binding its polo-box domain. These findings indicate the therapeutic potential of PLHSpT and peptides similarly targeted to surface receptors of cancer cells and to the functional domains of regulatory proteins.     

Protoplast Fusion of Lactobacillus casei

Lactobacillus casei ATCC 7469 was successfully converted to protoplasts by treatment with endo-7V-acetyl muramidase in sucrose phosphate buffer. For full hydrolysis of cell walls, a high concentration of sucrose and a cold shock were necessary. Mg²⁺ ions enhanced the stability of protoplasting cells. The cell wall regeneration of protoplasts was more effective on gelatin-induced regeneration medium than with the soft overlay method. The optimal concentration of gelatin was 2.5%. The frequency of regeneration was found to be about 6% for the protoplast prepared by enzyme treatment for 20 min. The mutants having streptomycin resistance and rifampicin resistance, as selection markers for the detection of fusion, were isolated by UV irradiation and NTG treatment. These mutants were stable for at least several transfers. Protoplast fusion was carried out using PEG (50% solution of polyethyleneglycol, M.W. 6,000). The frequency of protoplast fusion was found to be about 10^-5.     

Identification of Aniline-assimilating Bacteria

Twenty bacterial strains, grown on aniline as a sole source of carbon and nitrogen, and isolated from soil, were identified by morphological and biochemical tests, and cell wall analyses. Eight isolates were Rhodococcus erythropolis (Gray and Thornton) Goodfellow and Alderson, five were Pseudomonas maltophilia Hugh and Ryschenkow and seven were DAB (diaminobutyric acid)-type coryneform bacteria. The Rhodococcus spp. maintained the ability to assimilate aniline, but the pseudomonads and coryneform bacteria readily lost the ability, when grown in the absence of aniline.     

Effect of sorghum ethyl-acetate extract on benign prostatic hyperplasia induced by testosterone in Sprague–Dawley rats

ABSTRACT

Benign prostatic hyperplasia (BPH) is commonly observed in men > 50 years worldwide. Phytotherapy is one of the many treatment options. Sorghum (Sorghum bicolor L.) contains various health-improving phytochemicals with antioxidant and inhibitory activities on cell proliferation, both in vitro and in vivo. To confirm the effects of Donganme sorghum ethyl-acetate extract (DSEE) on BPH, we induced BPH in Spragye–Dawley rats using exogenous testosterone. We measured prostate weight, examined prostrates histopathologically, and analyzed mRNAs associated with male hormones and proteins associated with cell proliferation in the prostate. DSEE inhibited weight gain of the prostate; decreased mRNA expressions of androgen receptor and 5α-reductase II; and improved histopathological symptoms, the protein-expressed ratio of Bax/Bcl-2, and the oxidative status of BPH induced by testosterone in SD rats. Therefore, DSEE may have potential as a preventive or therapeutic agent against BPH.     

SESN2/sestrin2 suppresses sepsis by inducing mitophagy and inhibiting NLRP3 activation in macrophages

Proper regulation of mitophagy for mitochondrial homeostasis is important in various inflammatory diseases. However, the precise mechanisms by which mitophagy is activated to regulate inflammatory responses remain largely unknown. The NLRP3 (NLR family, pyrin domain containing 3) inflammasome serves as a platform that triggers the activation of CASP1 (caspase 1) and secretion of proinflammatory cytokines. Here, we demonstrate that SESN2 (sestrin 2), known as stress-inducible protein, suppresses prolonged NLRP3 inflammasome activation by clearance of damaged mitochondria through inducing mitophagy in macrophages. SESN2 plays a dual role in inducing mitophagy in response to inflammasome activation. First, SESN2 induces “mitochondrial priming” by marking mitochondria for recognition by the autophagic machinery. For mitochondrial preparing, SESN2 facilitates the perinuclear-clustering of mitochondria by mediating aggregation of SQSTM1 (sequestosome 1) and its binding to lysine 63 (Lys63)-linked ubiquitins on the mitochondrial surface. Second, SESN2 activates the specific autophagic machinery for degradation of primed mitochondria via an increase of ULK1 (unc-51 like kinase 1) protein levels. Moreover, increased SESN2 expression by extended LPS (lipopolysaccharide) stimulation is mediated by NOS2 (nitric oxide synthase 2, inducible)-mediated NO (nitric oxide) in macrophages. Thus, Sesn2-deficient mice displayed defective mitophagy, which resulted in hyperactivation of inflammasomes and increased mortality in 2 different sepsis models. Our findings define a unique regulatory mechanism of mitophagy activation for immunological homeostasis that protects the host from sepsis.