Intestinal Function and Reproductive Capacity of Tegel pullets in Response to Exogenous Oestrogen

The effects of varying levels of exogenous oestrogen (E₂) (0, 10 or 100µg E₂/kg BW) on the development of 18-week old pullets were tested over a 28-day period. The hormone had no significant effects on feed intake, body growth, feed conversion ratio or weight of the oviduct. Similarly, there were no significant effects of the hormone on egg production and egg weight but eggshell thickness and weight of shell per unit area were increased (P <0.05) at a lower level of administration (10µg E₂/kg BW), compared to the control and the highest level of hormone. The morphometry of the jejunal mucosa and some enzymes associated with Ca transport were similar between the three groups. Oestrogen treatment, however, intensely enhanced the expression of calbindin D_22K, although this was not quantified.     

Regulation of NADPH Oxidase Activity in Phagocytes: RELATIONSHIP BETWEEN FAD/NADPH BINDING AND OXIDASE COMPLEX ASSEMBLY*

The X⁺-linked chronic granulomatous disease (X⁺-CGD) variants are natural mutants characterized by defective NADPH oxidase activity but with normal Nox2 expression. According to the three-dimensional model of the cytosolic Nox2 domain, most of the X⁺-CGD mutations are located in/or close to the FAD/NADPH binding regions. A structure/function study of this domain was conducted in X⁺-CGD PLB-985 cells exactly mimicking 10 human variants: T341K, C369R, G408E, G408R, P415H, P415L, Δ507QKT509-HIWAinsert, C537R, L546P, and E568K. Diaphorase activity is defective in all these mutants. NADPH oxidase assembly is normal for P415H/P415L and T341K mutants where mutation occurs in the consensus sequences of NADPH- and FAD-binding sites, respectively. This is in accordance with their buried position in the three-dimensional model of the cytosolic Nox2 domain. FAD incorporation is abolished only in the T341K mutant explaining its absence of diaphorase activity. This demonstrates that NADPH oxidase assembly can occur without FAD incorporation. In addition, a defect of NADPH binding is a plausible explanation for the diaphorase activity inhibition in the P415H, P415L, and C537R mutants. In contrast, Cys-369, Gly-408, Leu-546, and Glu-568 are essential for NADPH oxidase complex assembly. However, according to their position in the three-dimensional model of the cytosolic domain of Nox2, only Cys-369 could be in direct contact with cytosolic factors during oxidase assembly. In addition, the defect in oxidase assembly observed in the C369R, G408E, G408R, and E568K mutants correlates with the lack of FAD incorporation. Thus, the NADPH oxidase assembly process and FAD incorporation are closely related events essential for the diaphorase activity of Nox2.     

High glucose/High Lipids impair vascular adiponectin function via inhibition of caveolin-1/AdipoR1 signalsome formation

Reduced levels of adiponectin (APN) contribute to cardiovascular injury in the diabetic population. Recent studies demonstrate elevated circulating APN levels are associated with endothelial dysfunction during pre-diabetes, suggesting the development of APN resistance. However, mechanisms leading to, and the role of, vascular APN resistance in endothelial dysfunction remain unidentified. The current study determined whether diabetes cause endothelial APN resistance, and by what mechanisms. Under high glucose/high lipids (HG/HL), APN-stimulated nitric oxide production by HUVEC was decreased, phosphorylation of eNOS, AMPK, and Akt was attenuated (P<0.01), and APN's anti-TNFα effect was blunted (P<0.01). APN receptor expression remained normal, whereas Cav1 expression was reduced in HG/HL cells (P<0.01). The AdipoR1/Cav1 signaling complex was dissociated in HG/HL cells. Knock-down of Cav1 inhibited APN's anti-oxidative and anti-inflammatory actions. Conversely, preventing HG/HL-induced Cav1 downregulation by Cav1 overexpression preserved APN signaling in HG/HL cells. Knock-in of a wild type Cav1 in Cav1 knock-down cells restored caveolae structure and rescued APN signaling. In contrast, knock-in of a mutated Cav1 scaffolding domain restored caveolae structure, but failed to rescue APN signaling in Cav1 knock-down cells. Finally, AdipoR1/Cav1 interaction was significantly reduced in diabetic vascular tissue, and the vasorelaxative response to APN was impaired in diabetic animals. The current study demonstrates for the first time the interaction between AdipoR1 and Cav1 is critical for adiponectin-mediated vascular signaling. The AdipoR1/Cav1 interaction is adversely affected by HG/HL, due largely to reduced Cav1 expression, supporting a potential mechanism for the development of APN resistance, contributing to diabetic endothelial dysfunction.     

Testing the stability of transfer functions

In dendroclimatology, testing the stability of transfer functions using cross-calibration verification (CCV) statistics is a common procedure. However, the frequently used statistics reduction of error (RE) and coefficient of efficiency (CE) merely assess the skill of reconstruction for the validation period, which does not necessarily reflect possibly instable regression parameters. Furthermore, the frequently used rigorous threshold of zero which sharply distinguishes between valid and invalid transfer functions is prone to an underestimation of instability. To overcome these drawbacks, we here introduce a new approach – the Bootstrapped Transfer Function Stability test (BTFS). BTFS relies on bootstrapped estimates of the change of model parameters (intercept, slope, and r²) between calibration and verification period as well as the bootstrapped significance of corresponding models. A comparison of BTFS, CCV and a bootstrapped CCV approach (BCCV) applied to 42,000 pseudo-proxy datasets with known properties revealed that BTFS responded more sensitively to instability compared to CCV and BCCV. BTFS performance was significantly affected by sample size (length of calibration period) and noise (explained variance between predictor and predictand). Nevertheless, BTFS performed superior with respect to the detection of instable transfer functions in comparison to CCV.     

Glycine neurotransmitter transporters: an update

Glycine accomplishes several functions as a transmitter in the central nervous system(CNS). As an inhibitory neurotransmitter, it participates in the processing of motor and sensory information that permits movement, vision, and audition. This action of glycine is mediated by the strychnine-sensitive glycine receptor, whose activation produces inhibitory post-synaptic potentials. In some areas of the CNS, glycine seems to be co-released with GABA, the main inhibitory amino acid neurotransmitter. In addition, glycine modulates excitatory neurotransmission by potentiating the action of glutamate at N-methyl-D-aspartate (NMDA) receptors. It is believed that the termination of the different synaptic actions of glycine is produced by rapid reuptake through two sodium-and-chloride-coupled transporters, GLYT1 and GLYT2, located in the plasma membrane of glial cells or pre-synaptic terminals, respectively. Glycine transporters may become major targets for therapeutic of pathological alterations in synaptic function. This article reviews recent progress on the study of the molecular heterogeneity, localization, function, structure, regulation and pharmacology of the glycine transporter     

Funktionsmorphologie des Exkretionsorgans des Spulwurms Ascaris lumbricoides L.

Zusammenfassung Das Seitenkanalsystem von Ascaris lumbricoides wurde elektronenmikroskopisch untersucht. Beim erwachsenen Tier erstreckt sich das in den lateralen Epidermisleisten eingebettete einzellige Organ vom Nervenring bis etwa zur Körpermitte. Im 2. Körperviertel besitzt es kein durchgehendes Kanallumen und erscheint degeneriert. In allen übrigen Bereichen (mit Ausnahme des Ausführungskanals) besitzt es den gleichen Aufbau aus zwei Schichten. Die das Kanallumen begrenzende innere Schicht enthält zahlreiche extraplasmatische Räume, von denen zumindest die am weitesten innen liegenden mit dem Kanallumen kommunizieren. Die äußere Zellmembran besitzt viele Einfaltungen, von denen einige weit in das Cytoplasma hineinragen. Der Gewebeanteil der lateralen Epidermisleisten, der dem Seitenkanalsystem unmittelbar anliegt, enthält sehr viele Interzellularräume, die ein zusammenhängendes Drainage-System bilden. Zur histochemischen Lokalisation von ATP-ase-Aktivität wurden Experimente durchgeführt. Die möglichen Mechanismen der Bildung der Exkretflüssigkeit werden diskutiert unter Berücksichtigung bereits veröffentlichter physiologischer Befunde.

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Ultrastructure and function of the excretory organ of Ascaris lumbricoides L. (Nematoda)

Summary The Excretory organ (H-system) of Ascaris lumbricoides has been investigated electronmicroscopically. In adult animals this single-cell-organ embedded in the lateral lines extends from the nerve ring to approximately the middle of the body.In the second quarter of the body it lacks a continuous canal lumen, and it seems to be degenerated. In all of the other regions (except the stem leading to the excretory pore) it consists of two zones. The inner zone lining the canal lumen contains several extraplasmatic spaces; at least those placed the farthest inside communicate with the canal lumen. The outer cell membrane shows many infoldings, some of which extend deeply into the cytoplasm. The tissue of the lateral line adjacent to the canal system contains very many intercellular spaces which build a coherent intracellular rainage-system. Experiments have been performed in order to localize the ATPase activity histochemically. Possible mechanisms for the forming of the excretory fluid are discussed under consideration of physiological results already published.

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Abkürzungen Ak Ausführungskanal - Bm Basalmembran - Cp Cytoplasmaplatten - lE linke Epidermisleiste - rE rechte Epidermisleiste - Ef Einfaltungen der äußeren Zellmembran - Fb Fibrillenbündel - Go Go Golgiapparat - Hg Hüllgewebe - Is lamelläre Interzellularsubstanz - Iz Interzellularraum - Kl Kanallumen - K Kutikula - Lh Leibeshöhle - Mu Muskelzelle - Mi Mitochondrien - Ms mittlerer Gewebestreifen (= Mittelstreifen) der Epidermisleiste - Mt Mikrotubuli - N Zellkern - No Nucleolus - Ne Nervenring - eP elektronendichte Partikel - sP sphärische Partikel - P Kernpore - Q Querbalken - epR extraplasmatischer Raum - Lho Längsholm - Mf Membranfusion - äS äußere Schicht des Seitenkanalsystems - iS innere Schicht der Längsholme - Sy syncytiale Cytoplasmamasse ohne Interzellularen - V Verzweigungskanal - iZ innere Zone um einen Verzweigungskanal Inauguraldissertation der Mathematisch-Naturwissenschaftlichen Fakultät der Freien Universität Berlin (gekürzt). Herrn Prof. Dr. G. Kümmel danke ich für die Anregung zu diesem Thema und für sein ständiges kritisches Interesse der Untersuchung, Frau C. S. Friedemann für die Anfertigung der Zeichnungen und Fräulein H. Schmidt für technische Assistenz.     

棕色田鼠与甘肃鼢鼠咀嚼肌结构和功能的比较

为了解棕色田鼠与甘肃鼢鼠对食物的适应机制, 对它们的咀嚼肌及相关的骨学特征做了比较解剖, 并运用生物力学原理分析下颌运动方式及食物加工过程的咀嚼效率。结果表明, 两个种的下颌的咀嚼均以水平面的前后向运动为主, 研磨加工植物纤维。相应地, 咀嚼肌、牙齿及相关的骨骼形态也具有一系列与此运动方式和功能相适应的结构特征, 如彼此平行的左右侧颊齿列、沟槽状的下颌关节窝以及咬肌的排列位置前移等。此外, 两个种具有几乎相同的门齿切割效率和臼齿咀嚼效率。两个种的上述相似特征与它们有着相似的食物结构是一致的。     

银杏叶中聚戊烯醇类化合物的研究进展

本文对银杏叶中聚戊烯醇类化合物的研究作了综述,主要包括它们的化学结 构、提取分离方法、光谱特征、分析方法、作用,以及多萜醇的合成等。并对其研究前景进 行了展望。     

可口革囊星虫肾管纤毛的分布及结构特征

为了解可口革囊星虫(Phascolosoma esculenta)肾管纤毛的结构特点及其功能,采用显微及亚显微技术观察研究了可口革囊星虫肾管纤毛的分布位置及形态结构特征。结果表明,肾管外膜多纤毛细胞表面簇生纤毛、内部柱状上皮细胞与立方上皮细胞游离面着生分散的纤毛,肾口内面也着生纤毛。纤毛结构由纤毛干、过渡区、基体及其纤毛小根组成;纤毛干由"9+2"结构的轴丝外被纤毛膜构成;纤毛干与基体之间为过渡区,中央微管终止于此,外周双联微管通过过渡区和基体的外周轴丝相连;基体呈圆筒状,为"9+0"结构;纤毛小根分长根和短根,均为基体发出的由微细原纤维组成的圆锥形结构,具间隔70 nm的明显横纹。肾管纤毛可能在促进体腔液流动、提高肾管对体腔液的过滤作用以及引导成熟精卵进入肾管等方面发挥作用。