Activation of AMPK by Bitter Melon Triterpenoids Involves CaMKKβ

We recently showed that bitter melon-derived triterpenoids (BMTs) activate AMPK and increase GLUT4 translocation to the plasma membrane in vitro, and improve glucose disposal in insulin resistant models in vivo. Here we interrogated the mechanism by which these novel compounds activate AMPK, a leading anti-diabetic drug target. BMTs did not activate AMPK directly in an allosteric manner as AMP or the Abbott compound (A-769662) does, nor did they activate AMPK by inhibiting cellular respiration like many commonly used anti-diabetic medications. BMTs increased AMPK activity in both L6 myotubes and LKB1-deficient HeLa cells by 20–35%. Incubation with the CaMKKβ inhibitor, STO-609, completely attenuated this effect suggesting a key role for CaMKKβ in this activation. Incubation of L6 myotubes with the calcium chelator EGTA-AM did not alter this activation suggesting that the BMT-dependent activation was Ca²⁺-independent. We therefore propose that CaMKKβ is a key upstream kinase for BMT-induced activation of AMPK.     

色氨酸残基在磷酸烯醇式丙酮酸羧化酶催化功能中的作用

在pH7.5条件下,用NBS对PEP羧化酶中色氨酸残基进行共价修饰表明,PEP羧化酶中48个色氨酸残基均能被NBS修饰。用邹承鲁图解法求得,其中4个残基为酶表现催化活性所必需的。 PEP羧化酶的变构效应剂G6P、Gly及Mal分别与酶预保温后,再经NBS修饰,前两种处理中,同样浓度的NBS所用修饰的色氨酸残基数和处理后的残存酶活与对照相比有很大的差异,而用Mal处理的,两者与对照相差无几。     

马齿苋叶片PEP羧化酶的分子特性

马齿苋叶片PEPCase由四个相同的亚基组成,亚基分子量为83kD。远紫外CD光谱分析表明,此酶含有36.6％α—螺旋结构。马齿苋叶片PEPCase可被G6P激活,但不能被Gly、Ser激活。G6P可防止酶的尿素变性和枯草杆菌蛋白酶的作用。这种保护效应与G6P诱导的酶构象变化有关。 从酶对低温、高温及尿素的反应来看,马齿苋叶片PEPCase的稳定性高于高粱叶片PEP—Case,两者的免疫特性和电泳特性亦不同。     

下丘脑室旁核加压素能神经元参与电针刺激对实验性内脏痛的抑制

本实验采用内脏痛的实验模型,探讨室旁核中的加压素在针刺抑制内脏痛中的作用。实验结果如下:(1)大鼠在在射酒石酸锑钾(0.1％,10ml/kg,i.p.)后,出现可定量的扭体反应,能作为观察内脏痛的客观指标。(2)电针对内脏痛有抑制效应,即具有镇痛作用。(3)电刺激室旁核,能加强电针对内脏痛的抑制效应,损毁室旁核,则此抑制效应基本消失。(4)脑室注射加压素抗血清(14μl)或加压素拮抗剂[d(CH_2)_5Tyr(Me)-AVP,500ng/5μl]都能明显减弱电针的抑制效应。(5)腹腔注射加压素拮抗剂(10μg/kg),不能翻转电针的抑制效应。上述实验结果表明,下丘脑室旁核的加压素能神经元参与了电针刺激对实验性内脏痛的抑制。     

春小麦胚芽伸长过程中渗透调节与能量代谢

本文用PEG模拟水分亏缺对春小麦红芒麦和绵阳11号胚芽伸长过程中生长、膨压、渗透势、水势和渗透调节能力与ATP含量、能荷变化及能量代谢间的关系进行了研究。结果表明,通过降低能荷,改变分解代谢与合成代谢的比率,使渗透调节物质积累,增加了幼苗的吸水能力,从而使其在一定的ATP能量水平上维持缓慢生长;抗旱品种红芒麦在水分亏缺下成苗速率较快,能保持一定的ATP能量水平和能荷值,渗透调节和吸水能力都比较强。     

降解嘌呤核苷乳酸菌的筛选及益生特性探索

【背景】高尿酸血症是人体内嘌呤代谢紊乱导致的一种慢性代谢疾病,利用乳酸菌降解嘌呤类物质是辅助治疗高尿酸血症的新方法。【目的】筛选高效降解嘌呤核苷的乳酸菌并对其益生特性进行研究。【方法】利用HPLC法评价乳酸菌对肌苷、鸟苷的降解效果。通过药敏性试验、体外耐受性试验及细胞黏附试验研究目标菌株的益生特性。【结果】筛选出一株发酵乳杆菌(Lactobacillus fermentum) SR2-6,对肌苷和鸟苷的降解率分别为99.26%和98.85%。该菌株对青霉素、氯霉素等5种常见抗生素不具备耐药性,在pH 2.0环境下处理4 h后菌株的存活率为76.51%,在饱腹状态下的人工肠液模拟消化4 h后活菌数仍能达到6.85 lg (CFU/mL),对Caco-2细胞的黏附数为(52.29±15.14) CFU/cell。【结论】发酵乳杆菌SR2-6能够高效降解肌苷和鸟苷且具有优良的益生特性,是预防和治疗高尿酸血症的潜在优势菌株,可作为优势菌种资源应用于相关功能产品的开发。     

PDGF-AA activates AKT and ERK signaling for testicular interstitial Leydig cell growth via primary cilia

Testes control the development of male reproductive system. The testicular interstitial Leydig cells (Leydig cells) synthesize testosterone for promoting spermatogenesis and secondary sexual characteristics. Type A platelet-derived growth factor (PDGF-AA) is one of the most important growth factors in regulating Leydig cell growth and function. Knockout of PDGF-AA or its congenital receptor PDGFR-α leads to poor testicular development caused by reducing Leydig cell numbers, supporting PDGF-AA/PDGFR-α signaling regulates Leydig cell development. Primary cilium is a cellular antenna that functions as an integrative platform to transduce extracellular signaling for proper development and differentiation. Several receptors including PDGFR-α are observed on primary cilia for initiating signaling cascades in distinct cell types. Here we showed that PDGF-AA/PDGFR-α signaling promoted Leydig cells growth, migration, and invasion via primary cilia. Upon PDGF-AA treatment, AKT and ERK signaling were activated to regulate these cellular events. Interestingly, active AKT and ERK were detected around the base of primary cilia. Depletion of ciliary genes (IFT88 and CEP164) alleviated PDGF-AA-activated AKT and ERK, thus reducing Leydig cell growth, migration, and invasion. Thus, our study not only reveals the function of PDGF-AA/PDGFR-α signaling in maintaining testicular physiology but also uncovers the role of primary cilium and downstream signaling in regulating Leydig cell development.     

干旱胁迫下红砂幼苗非结构性碳水化合物动态变化特征

该试验以荒漠区主要建群种红砂幼苗为研究对象,设置适宜水分(CK)、轻度干旱(MD)、中度干旱(SD)和重度干旱(VSD)4个胁迫处理(即田间持水量的80%、60%、40%和20%),采用盆栽控水试验,分别测定干旱胁迫15、30、45和60 d时红砂幼苗的叶、茎、粗根和细根中非结构碳水化合物(NSC)及其组分的含量,分析不同胁迫强度下不同干旱持续时间红砂幼苗NSC的动态变化及各组分差异,以揭示红砂NSC对干旱胁迫的响应机制。结果表明:(1)干旱胁迫强度和胁迫持续时间对红砂幼苗不同器官NSC及其组分均有显著影响,其中胁迫持续时间对NSC动态变化的影响尤为显著。(2)干旱胁迫初期,红砂叶中的NSC含量呈下降趋势,而茎中的NSC含量呈上升趋势,粗根和细根中NSC含量在各胁迫处理下基本保持稳定。(3)干旱胁迫后期,红砂叶和茎中的可溶性糖、淀粉和NSC含量逐渐增加,而粗根和细根中的淀粉和NSC含量呈下降趋势(中度干旱除外),且这一时期重度干旱处理下各器官可溶性糖和NSC的含量明显高于CK。研究发现,重度干旱胁迫能显著诱导提高红砂幼苗不同器官中的NSC含量,并通过分解根中淀粉和增加叶片中可溶性糖含量的方式来调节细胞渗透势平衡,以维持细胞活力,进而保持红砂在干旱胁迫后期的存活。     

PRIMORDIAL GERM CELL-DERIVED MOUSE EMBRYONIC GERM (EG) CELLSIN VITRORESEMBLE UNDIFFERENTIATED STEM CELLS WITH RESPECT TO DIFFERENTIATION CAPACITY AND CELL CYCLE DISTRIBUTION

Embryonic germ (EG) cells of line EG-1 derived from mouse primordial germ cells were investigated for theirin vitrodifferentiation capacity. By cultivation as embryo-like aggregates EG-1 cells differentiated into cardiac, skeletal muscle and neuronal cells accompanied by the expression of tissue-specific genes and proteins as shown by RT-PCR analysis and indirect immunofluorescence. In comparison to embryonic stem (ES) cells of line D3 the efficiency of differentiation into cardiac and muscle cells was comparatively low, whereas spontaneous neuronal differentiation was more efficient than in D3 cells. Furthermore, the distribution of cell cycle phases as a parameter for the differentiation state was analysed in undifferentiated EG cells and ES cells and compared to data obtained for embryonic carcinoma (EC) cells of line P19 and differentiated, epithelioid EPI-7 cells. Flow cytometric analysis revealed similar cell cycle phase distributions in EG, EC and ES cells. In contrast, the somatic differentiated EPI-7 cells showed a longer G₁-phase and shorter S- and G₂/M-phases. Together, our results demonstrate that the differentiation state and capacity of EG cellsin vitroresemble that of totipotent ES cells.