Bronchoconstriction Induces TGF-β Release and Airway Remodelling in Guinea Pig Lung Slices

Airway remodelling, including smooth muscle remodelling, is a primary cause of airflow limitation in asthma. Recent evidence links bronchoconstriction to airway remodelling in asthma. The mechanisms involved are poorly understood. A possible player is the multifunctional cytokine TGF-β, which plays an important role in airway remodelling. Guinea pig lung slices were used as an in vitro model to investigate mechanisms involved in bronchoconstriction-induced airway remodelling. To address this aim, mechanical effects of bronchoconstricting stimuli on contractile protein expression and TGF-β release were investigated. Lung slices were viable for at least 48 h. Both methacholine and TGF-β₁ augmented the expression of contractile proteins (sm-α-actin, sm-myosin, calponin) after 48 h. Confocal fluorescence microscopy showed that increased sm-myosin expression was enhanced in the peripheral airways and the central airways. Mechanistic studies demonstrated that methacholine-induced bronchoconstriction mediated the release of biologically active TGF-β, which caused the increased contractile protein expression, as inhibition of actin polymerization (latrunculin A) or TGF-β receptor kinase (SB431542) prevented the methacholine effects, whereas other bronchoconstricting agents (histamine and KCl) mimicked the effects of methacholine. Collectively, bronchoconstriction promotes the release of TGF-β, which induces airway smooth muscle remodelling. This study shows that lung slices are a useful in vitro model to study mechanisms involved in airway remodelling.     

Understanding Miro GTPases: Implications in the Treatment of Neurodegenerative Disorders

The Miro GTPases represent an unusual subgroup of the Ras superfamily and have recently emerged as important mediators of mitochondrial dynamics and for maintaining neuronal health. It is now well-established that these enzymes act as essential components of a Ca²⁺-sensitive motor complex, facilitating the transport of mitochondria along microtubules in several cell types, including dopaminergic neurons. The Miros appear to be critical for both anterograde and retrograde mitochondrial transport in axons and dendrites, both of which are considered essential for neuronal health. Furthermore, the Miros may be significantly involved in the development of several serious pathological processes, including the development of neurodegenerative and psychiatric disorders. In this review, we discuss the molecular structure and known mitochondrial functions of the Miro GTPases in humans and other organisms, in the context of neurodegenerative disease. Finally, we consider the potential human Miros hold as novel therapeutic targets for the treatment of such disease.     

Characterization and Physiological Importance of a Novel Cell Cycle Regulated Protein Kinase inXenopus laevisOocytes That Phosphorylates Cyclin B2

We have partially purified a specific cyclin B2 kinase (cyk) from prophase oocytes ofXenopus laevisafter an ATP-γ-S activation step. Phosphopeptide analysis identified Ser53 as the majorin vitrophosphorylation site for cyk in cyclin B2. Using a synthetic peptide derived from cyclin B2 encompassing Ser53 (cyktide) as a substrate, cyk was shown to be activated during progesterone-induced maturation, with a peak of activity between 40 and 50% maturation. A sustained high cyk activity was observed in oscillating egg extracts. Microinjection of cyk-phosphorylated cyclin B2 into prophase oocytes accelerated progesterone-induced maturation by about 2 h, indicating that cyclin B2 is a relevant substrate for cyk and that the function of cyk is situated upstream of cdc2-cyclin B activation. Microinjection of cyk-phosphorylated cyktide or a combination of cyk and cyclin B1 into G₂fibroblasts induced significant changes in cell morphology, reminiscent of a premature prophase-like phenotype. Similarly, addition of cyk-phosphorylated cyktide in cyclin B1-dependent interphase extracts resulted in histone H1 kinase activation.     

Frostresistenzprüfungen an keimenden Kernobstsamen

Ohne ZusammenfassungMit 3 Textabbildungen.     

Quantitative Untersuchung der Osteonverteilung im Extremitätenskelet eines 43jährigen Mannes

Zusammenfassung Die Beschreibung der Struktur 2. Ordnung baut auf einer Klassifizierung der Strukturen 3. Ordnung, Osteone und Tangentiallamellen, auf (Knese, Voges und Ritschl 1954). Um die Zusammenlagerung der Osteone mit verschiedenen Merkmalen wie Form, Größe und Steigungsfolge am einzelnen Ort zu erfassen, wird das Lochkartenverfahren benutzt. Die Besonderheiten dieses Verfahrens, das sich von der üblichen Beschreibung sowie der Zahlenstatistik unterscheidet, bzw. eine Kombination beider darstellt, werden diskutiert. Es wird darauf hingewiesen, daß die Verwendung des Lochkartenverfahrens die Möglichkeit gibt, eine unübersichtliche Ansammlung sehr ähnlicher Gebilde in ihren einzelnen Bestandteilen zu differenzieren.Typen einer Struktur 2. Ordnung, die an verschiedenen Skeletelementen wiederkehren, existieren nicht. Es ist daraus zu schließen, daß jedes Skeletstück in seinen verschiedenen Anteilen einen individuellen Bau besitzt. Damit kann aber auch nicht mit einem gleichartigen Spannungsgefüge an verschiedenen Skeletstücken gerechnet werden. Die Verteilung der Strukturen ist als Funktion (im mathematischen Sinn) des Querschnittes anzusehen. Asymmetrische Osteone haben Verteilungsschwerpunkte an den Flächen, Runde und Schrägschnitte an den Kanten. In einem Skeletstück herrscht eine Steigungsfolge vor. Gleichartige Wicklungen finden sich zum Teil an gegenüberliegenden Flächen. Im einzelnen ist die Verteilung der Steigungsfolgen über den Querschnitt ähnlich wie die der Asymmetrierichtungen sehr verwickelt.Ausgeführt mit Unterstützung der Deutschen Forschungsgemeinschaft.     

Role of biotin-containing membranes and nuclear distribution in differentiating human endometrial cells

Human Ishikawa endometrial cells form domes when confluent monolayers are stimulated with fresh fetal bovine serum. Extensive structural and biochemical changes have been detected during the approximately 30 h differentiation period. The earliest detectable change involves the formation of multinucleated structures and the appearance of “granules” that stain for biotin within those structures. Nuclei become associated with each other and are ultimately enclosed within a biotin-containing membrane. Aggregated membrane-sheathed nuclei and the cells containing them begin to elevate from the dish as biotin staining becomes apparent in apical membranes. The elevated structures are called predomes and consist of one or more very large cells containing the sheathed nuclei. Apical membranes of these unusual cells extend far out into the medium in structures that resemble endometrial pinopods. A lumen under the elevated cells fills with transcytosed fluid. As differentiation proceeds, highly concentrated chromatin material that was flattened against apical and lateral membranes of the predome cells begins to disperse. Small mononuclear cells evolve from larger predome cells. Apical membranes of predome and dome cells continue to stain for biotin. Gel electrophoresis of SDS-solubilized biotin-containing membranes, followed by Western blot analysis using avidin-linked peroxidase, resulted in three stained bands with molecular weights similar to those of the mitochondrial carboxylases: propionyl carboxylase, methylmalonyl carboxylase, and pyruvate carboxylase. J. Cell. Biochem. 71:400–415, 1998. © 1998 Wiley-Liss, Inc.