Hypoxic vasoconstriction of partial muscular intra-acinar pulmonary arteries in murine precision cut lung slices
- 8.2k Downloads
Acute alveolar hypoxia causes pulmonary vasoconstriction (HPV) which serves to match lung perfusion to ventilation. The underlying mechanisms are not fully resolved yet. The major vascular segment contributing to HPV, the intra-acinar artery, is mostly located in that part of the lung that cannot be selectively reached by the presently available techniques, e.g. hemodynamic studies of isolated perfused lungs, recordings from dissected proximal arterial segments or analysis of subpleural vessels. The aim of the present study was to establish a model which allows the investigation of HPV and its underlying mechanisms in small intra-acinar arteries.
Intra-acinar arteries of the mouse lung were studied in 200 μm thick precision-cut lung slices (PCLS). The organisation of the muscle coat of these vessels was characterized by α-smooth muscle actin immunohistochemistry. Basic features of intra-acinar HPV were characterized, and then the impact of reactive oxygen species (ROS) scavengers, inhibitors of the respiratory chain and Krebs cycle metabolites was analysed.
Intra-acinar arteries are equipped with a discontinuous spiral of α-smooth muscle actin-immunoreactive cells. They exhibit a monophasic HPV (medium gassed with 1% O2) that started to fade after 40 min and was lost after 80 min. This HPV, but not vasoconstriction induced by the thromboxane analogue U46619, was effectively blocked by nitro blue tetrazolium and diphenyleniodonium, indicating the involvement of ROS and flavoproteins. Inhibition of mitochondrial complexes II (3-nitropropionic acid, thenoyltrifluoroacetone) and III (antimycin A) specifically interfered with HPV, whereas blockade of complex IV (sodium azide) unspecifically inhibited both HPV and U46619-induced constriction. Succinate blocked HPV whereas fumarate had minor effects on vasoconstriction.
This study establishes the first model for investigation of basic characteristics of HPV directly in intra-acinar murine pulmonary vessels. The data are consistent with a critical involvement of ROS, flavoproteins, and of mitochondrial complexes II and III in intra-acinar HPV. In view of the lack of specificity of any of the classical inhibitors used in such types of experiments, validation awaits the use of appropriate knockout strains and siRNA interference, for which the present model represents a well-suited approach.
KeywordsFumarate U46619 Luminal Area Fumarate Reductase Alveolar Duct
Acute alveolar hypoxia causes pulmonary vasoconstriction . This hypoxic pulmonary vasoconstriction (HPV) directs blood flow towards well ventilated areas of the lung, and, hence, optimizes gas exchange by matching lung perfusion to ventilation. This principally beneficial reflex may turn into a pathogenetic mechanism under conditions of chronic alveolar hypoxia resulting in pulmonary hypertension characterized by remodelling of the pulmonary vasculature and right ventricular hypertrophy. Studies aimed to elucidate the molecular mechanisms underlying acute HPV identified several candidates that may serve as the initial cellular oxygen sensor(s). These include components of the mitochondrial respiratory chain, non-mitochondrial enzymes generating reactive oxygen species (ROS), and plasmalemmal potassium channels . However, partly conflicting data have been obtained and a consensus has not been reached yet.
Still, it is well accepted that, along the pulmonary vascular bed, there is a marked regional diversity in reactivity to hypoxia [3, 4]. In the rat, for example, conduit pulmonary artery rings respond to hypoxia after an initial small constriction with a relaxation below baseline, whereas rings from vessels with less than 300 μm in external diameter respond by a monophasic constriction . Thus, at least part of the observed incoherence of data between studies is likely to be due to investigation of different arterial segments and to the use of different experimental approaches. Hemodynamic studies of perfused lungs [5, 6, 7] provide valuable information in that they most closely match the clinical situation, but the differential contributions of the various segments of the pulmonary vascular tree can hardly be discriminated. Electrophysiological and force recordings of isolated pulmonary artery segments or of myocytes dissociated from them are primarily aimed to be conducted on small or resistance vessels. Sizes reported for such vessels isolated from rat lung range from <300μm in external diameter  to 490 μm in inner diameter . Arteries of that size are fully muscular and usually accompany the conductive airway in its adventitial sheath, although some supernumerary branches that directly pass to the alveolar region immediately adjacent to the bronchoarterial sheath reach this diameter .
Micropuncture techniques of subpleural vessels as introduced by Bhattacharya and Staub , however, located the most significant drop in perfusion pressure to much more peripheral vascular segments in many species (for review, see ) with a particular sensitivity to hypoxia of the arterial part of the microcirculation . Visualization of rat subpleural microvessels by real-time confocal laser scanning luminescence microscopy localized highest sensitivity to hypoxia to immediate pre-capillary (diameter: 20–30 μm) vascular segments . Along the course of smallest pulmonary arteries towards the alveolar capillaries, their muscle coat first becomes incomplete with smooth muscle cells typically being present as a spiral before they vanish and are replaced by a discontinuous layer of intermediate cells and, finally, by pericytes [13, 14]. These non-muscular, partially muscular and the thinnest muscular arterial segments are located within the pulmonary acinus, i.e. the region beyond the terminal bronchiolus which represents the basic ventilatory unit . In contrast to the resistance arteries running in the bronchoarterial sheaths, these intra-acinar arteries lack an adventitial layer and are immediately flanked by alveoli whose septa are attached to the vascular elastic lamina. Hence, they are exquisitely located to monitor alveolar oxygen tension within that particular ventilatory unit that they perfuse, and therefore their reactions to reduced oxygen are of particular interest. Anatomically, partial muscular arteries are positioned between the smallest resistance vessels that so far have been dissected for physiological experiments and the surface-near microvessels that can sufficiently be reached by subpleural micropuncture or confocal laser scanning luminescence. Consequently, their responses to changes in oxygen tension have not been directly investigated yet.
In order to bridge that gap we adopted a method that was originally introduced for videomorphometric analysis of airway constriction in precision-cut lung slices (PCLS)  and is principally also suited to monitor vascular reactivity, ROS and NO production, and electrophysiological properties of vascular cells [16, 17, 18, 19]. In view of further extension of this technique to genetically engineered mouse strains (cf. [19, 20, 21]) we performed this study on murine PCLS. Since the general architecture of the pulmonary vasculature in this species is less known than in rat (cf. [13, 14, 22]) we first conducted a morphological and immunohistochemical survey study on murine PCLS to briefly characterize pre- and intra-acinar vessels. This enabled us to subsequently identify intra-acinar arteries in the videomorphometric set-up. In a recent PCLS study of murine small (inner diameter: 20–150 μm) vessels we obtained evidence for hypoxia-induced ROS generation and for an essential role of complex II of the respiratory chain in this process . Following this line, we used the newly developed approach to assess the impact of inhibition of respiratory chain complexes and of ROS production on HPV in murine intra-acinar arteries.
9,11-Dideoxy-11α,9α-epoxy-methanoprostaglandin F2α (U46619; final conc.: 10 μM), nitro blue tetrazolium (NBT; final conc.: 500 nM), diphenyleniodonium (DPI; final conc.: 10 μM), 3-nitropropionic acid (3-NPA; final conc.: 5 mM), thenoyltrifluoroacetone (TTFA; final conc.: 50 μM), antimycin A (AA; final conc.: 3 μg/ml), sodium azide (NaN3; final conc.: 1 mM), succinate, fumarate, and malic acid (final conc. of each: 15 mM) were purchased from Sigma Aldrich (Deisenhofen, Germany). Sodium nitroprusside (Nipruss; final conc.: 30 μM) was obtained from Schwarz Pharma GmbH Deutschland (Monheim, Germany).
Preparation of PCLS of murine lungs
PCLS were prepared according to protocols described by Martin et al.  and Pfaff et al. . Briefly, 8–12 weeks old FVB mice (Harlan-Winkelmann, Borchen, Germany) were killed by cervical dislocation and the blood was removed from the pulmonary vasculature by in situ perfusion with 37°C HEPES-Ringer buffer (10 mM HEPES, 136.4 mM NaCl, 5.6 mM KCl, 1 mM MgCl2, 2.2 mM CaCl2, 11 mM glucose, pH 7.4) containing heparin (250 I.U./ml) and penicillin/streptomycin (1%) via the right ventricle. Subsequently, the airways were filled via the cannulated trachea with 1.5% low melting point agarose (Bio-Rad Laboratories GmbH, Munich, Germany) dissolved in HEPES-Ringer buffer. Lungs and heart were removed en bloc and transferred into ice-cold HEPES-Ringer buffer to solidify the agarose. The lungs were cut into 200 μm thick slices using a vibratome (VT1000S, Leica, Bensheim, Germany). The agarose was removed by incubation in phenolred-free minimal essential medium (MEM) continuously gassed with 21% O2, 5% CO2, 74% N2 for at least 2 h at 37°C.
Immunohistochemistry of PCLS
For examination of the morphology of pulmonary vessels, 200 μm thick PCLS were cut from the left lobe of 4 animals as described above except for two changes in the protocol. 1) The lungs were filled with 3% low melting point agarose to facilitate cutting of bronchi that were oriented longitudinally to the cutting direction. 2) The sections were cut in the frontal plane to visualize better the course of blood vessels. After removing the agarose, the sections were fixed for 20 min in ice-cold acetone and washed repeatedly in 0.1 M phosphate buffer. Sections were covered for 1 h with blocking medium (10% normal horse serum, 0.5% Tween 20, 0.5% bovine serum albumin in PBS) followed by overnight incubation with a monoclonal FITC-labelled anti-α-smooth muscle actin (αSMA) antibody (1:500, clone 1A4, Sigma Aldrich). The sections were then washed in PBS and coverslipped in carbonate-buffered glycerol, pH 8.6. The morphology of arteries and veins was evaluated with a Zeiss Axioplan 2 epifluorescence microscope (Jena, Germany).
To assess the morphology of the muscular coat of vessels that were investigated in a videomorphometric analysis, in 23 PCLS the position of the examined vessel was documented at the end of an experiment. Phase contrast images were taken at different magnifications and the slices were subsequently processed for immunohistochemistry as described above. After the labelling, the individual vessel was identified and its α SMA-immunoreactivity was evaluated using either an epifluorescence microscope or a confocal laser scanning microscope (TCS-SP2 AOBS, Leica).
Videomorphometric analysis of PCLS
Studies on PCLS were performed in a flow-through superfusion chamber (Hugo Sachs Elektronik, March-Hugstetten, Germany) filled with phenolred-free MEM. The slices were held in place in the chamber with nylon strings that were connected to a platinum ring. At the beginning of each experiment the capability of the vessel to contract in response to the thromboxane analogue U46619 and to dilate after application of the NO donor Nipruss was checked. The flow rates were 0.7 ml/min during incubation with normoxic (21% O2, 5% CO2, 74% N2) or hypoxic medium (1% O2, 5% CO2, 94% N2) and 6 ml/min for washing steps. Immediately before feeding the normoxic and hypoxic gassed MEM into the perfusion chamber oxygen partial pressure (pO2) was analysed in a blood gas analyser (ABL510, Radiometer, Copenhagen, Denmark). The application of U46619 and Nipruss was performed at flow arrest, the medium containing the other substances was added at low flow rates (0.7 ml/min). The superfusion chamber was mounted on an inverted microscope (Leica), and images of intrapulmonary vessels with inner diameters between 20 and 150 μm were recorded using a CCD-camera (Stemmer Imaging, Puchheim, Germany). Pictures were taken every 2 min using the Optimas 6.5 software (Stemmer Imaging). Changes of the vascular luminal area were evaluated by lining the inner boundaries by hand. The area of the vascular lumen at the beginning of the experiment was set as 100%, and vasoconstriction and -dilatation were expressed as relative decrease or increase of this area.
For a clear graphic presentation of the effects of various substances on hypoxia- and the following U46619-induced pulmonary vasoconstriction, the value obtained immediately before exposure to reduced oxygen was set as 100%. The initial phase of the experiments which tested the viability of the vessels by application of U46619 and Nipruss was not integrated in the graphs unless explicitly stated.
Data are presented as means ± standard error of the mean (SEM) of 5–11 intra-acinar arteries per condition. A single vessel per PCLS was analysed. PCLS for each experimental condition were obtained from 3–5 mice. Statistical analysis was performed using SPSS 11.5.1. Differences among experimental groups were analyzed with the Kruskal-Wallis- followed by the Mann-Whitney-test, with p ≤ 0.05 being considered significant, and p ≤ 0.01 highly significant.
α-Smooth muscle actin immunohistochemistry
Pulmonary arteries and their discrimination from pulmonary veins
PCLS represent a suitable model for studying HPV of partially muscular intra-acinar arteries
To clarify whether these vessels still exhibit HPV, PCLS were exposed to hypoxic gassed medium. The pO2 of this medium (gassed previously for about 2 h with 1% O2) was reduced to 40 mmHg. We observed an immediately starting, progressive monophasic reduction of the luminal area which reached its maximum after about 20–30 min (40% reduction of the luminal area) and slowly started to fade after 40 min. On average, luminal area returned to initial values after 80 min of exposure to hypoxia, but individual vessels maintained HPV up to 120 min (Fig. 4). Longer periods of hypoxia were not tested. No changes in the luminal area occurred in control incubations with normoxic gassed medium (pO2: 160 mmHg). Subsequent incubation of the PCLS with U46619 resulted again in a marked vasoconstriction, regardless whether the PCLS had been previously exposed to normoxic or to hypoxic medium (Fig. 4).
After videomorphometric analysis, PCLS were stained for αSMA as marker for smooth muscle cells. With the aid of low magnification pictures taken at the end of the videomorphometric experiments, vessels were readily re-identified. All of the vessels from which responses to reduced oxygen tension have been recorded before were partially muscular intra-acinar arteries with a relatively thin, discontinuous layer of αSMA-immunoreactive cells typically arranged in a spiral (Fig. 4G, H).
Intra-acinar HPV requires ROS
Intra-acinar HPV requires a flavoprotein
As shown in Fig. 5B, preloading of PCLS with the flavoprotein inhibitor DPI resulted in significant vasoconstriction of intra-acinar arteries under normoxic conditions. This vasoconstriction reversed to dilatation under hypoxia, and HPV was not observed. The capability to respond to U46619 after hypoxic exposure was unimpaired by DPI (Fig. 5B).
Intra-acinar HPV demands functional mitochondrial complex II
Application of another inhibitor of complex II, TTFA, distinctly decelerated HPV (Fig. 6B). Ten minutes after onset of hypoxic exposure, the TTFA-treated vessels still exhibited no vasoconstriction whereas the luminal area of the control group was reduced by 20% (difference between groups: p = 0.024). Thereafter, HPV occurred in the TTFA group with an overall trend towards diminished vasoconstriction compared to the control vessels. The difference between both groups was significant at the end of exposure to hypoxia (p = 0.04). Both groups reacted identically to subsequent application of U46619 (Fig. 6B).
Succinate, the substrate of succinate dehydrogenase and the product of fumarate reductase activity of complex II, prevents intra-acinar HPV
Corresponding experiments with fumarate instead of succinate revealed only weak effects on HPV. The response to hypoxia was delayed, but reached the same degree of vasoconstriction as the untreated control after 30 min (Fig. 7B). Fumarate did not interfere with U46619-induced constriction.
Malate almost entirely prevented HPV, but also diminished markedly the U46619-induced response, indicating general effects of malate on intra-acinar vasoconstriction (Fig. 7C).
Intra-acinar HPV requires functional mitochondrial complex III
Inhibition of complex IV generally affects intra-acinar vasoconstriction
Administration of the complex IV inhibitor NaN3 abolished HPV and, instead, intra-acinar vessels exhibited slight dilatation (Fig. 8B). Vasoconstriction induced by U46619 was distinctly diminished by application of NaN3 (reduction of luminal area 40% versus 77% in the control group; p = 0.011) (Fig. 8B).
Intra-acinar murine pulmonary vessels and their constrictor response to hypoxia
With respect to the general structural features that could be evaluated from α SMA-labelled PCLS, murine intrapulmonary arteries show a striking resemblance to that reported for the rat (cf. review by ). These similarities include nearly rectangular branching of supernumerary arteries, and step-by-step transition of fully muscular small arteries first to segments where the muscle layer is incomplete with the muscle typically being present as a spiral, and finally to non-muscular segments. Judged from anatomical position, size, and wall thickness, intra-acinar vessels could be identified in living murine PCLS. Despite the fact that they, typically, were only partially muscular they showed a long lasting monophasic constriction in response to hypoxia. In the rat, the partially muscular intra-acinar arteries contain, in addition to the typical vascular smooth muscle cells, so-called "intermediate" cells which lie internal to the elastic membrane. They are considered as contractile cells as well, and as precursors of smooth muscle cells under conditions of vascular remodelling [14, 22]. In the immediate precapillary, non-muscular region, intermediate cells are replaced by pericytes which are also interpreted as contractile smooth muscle precursors [23, 24]. While data on intermediate cells in the murine lung are lacking, pulmonary pericytes have been identified and reported to be α SMA-negative or stain only weakly at maturity [25, 26]. Hence, the distinct HPV of partially muscular intra-acinar arterial segments, i.e. those with incomplete α SMA-immunolabelling, may not only rely on α SMA-positive smooth muscle cells but also on additional contractile cells as well.
Pulmonary artery pressure curves recorded from isolated perfused hypoxic murine lungs reach a peak as early as after 6 min, are biphasic and do not return to basal levels after 3 h even when ventilation is switched to normoxic conditions [27, 28, 29]. In contrast, HPV of intra-acinar arteries in PCLS developed slower, was monophasic, and was fully lost after 80 min even at continuing hypoxia. An obvious major difference between these experimental set-ups is the lack of shear-stress acting upon the endothelium in the PCLS model. In perfused vessels, acute HPV leads to a rise in shear-stress thereby inducing secondary mechanisms such as NO release [4, 5, 30]. Shear-stress alone, however, shall not fully account for the biphasic versus monophasic difference in HPV, because a biphasic response can also be recorded from non-perfused isolated pulmonary artery rings mounted in a vessel myograph (rat: ). Still, this type of preparation differs from PCLS in two major aspects beyond that of a species difference: First, it records tension under isometric conditions whereas the latter records metric changes (luminal area) under isotonic conditions, assuming that the force created by stretching the elastic alveolar attachments during vasoconstriction is negligible when the lung is collapsed. Second, resistance vessels analysed by myography, although being small, are still located distinctly upstream to the intra-acinar vessels monitored in PCLS. Thus, it remains to be determined whether a monophasic HPV is an exclusive characteristic of intra-acinar vessels or whether it is also a basic feature of other segments of the pulmonary vasculature when shear-stress and other secondary events are eliminated.
ROS in intra-acinar HPV
In a preceding study of murine PCLS exposed to hypoxia we observed increased ROS production in small (inner diameter: 20–150 μm) intrapulmonary arteries which required functional complex II of the mitochondrial respiratory chain and was also sensitive to blockade of complex III . The present data provide evidence that these hypoxia-induced events are directly linked to the contractile response of intra-acinar vessels. Evidence for a hypoxia-induced ROS production in pulmonary vessels has been provided earlier by several other approaches (e.g. [31, 32]), although there are also conflicting data (e.g. ). This controversy is extensively discussed in two recent reviews [34, 35], and it is likely that at least part of the inconsistencies between studies is due to investigation of different arterial segments and use of different experimental approaches. With respect to the effects of exogenously applied ROS, e.g. H2O2, under normoxia and of ROS scavengers under hypoxia, there is less diversity reported: 1) H2O2 constricts the pulmonary circulation during normoxia , 2) inhibition of the endogenous H2O2 scavenger, catalase, augments HPV , and 3) the ROS scavenger NBT prevents HPV in isolated perfused rabbit lungs  and completely abrogated intra-acinar HPV in our experiments. Also, DPI, a broad flavoprotein inhibitor that suppresses ROS production in many systems including murine PCLS [18, 38], blocks HPV in perfused rabbit lungs , pulmonary artery rings from cats , and in our murine PCLS model. Hence, the present data are consistent with the view that augmented ROS production is required for HPV of intra-acinar arteries.
Mitochondrial complexes II and III in intra-acinar HPV
The mitochondrial electron transport chain is currently considered as the major, although not necessarily exclusive, source of hypoxia-induced altered ROS production [34, 35]. Particular attention has been paid to complex III which receives electrons from ubiquinol generated either at complex I or complex II. Inhibition of complex III abolishes or attenuates HPV in each model investigated so far [7, 8, 32, 33] including our present study on intra-acinar vessels in murine PCLS. Some uncertainty, however, has arisen as to the specificity of this effect for hypoxia-induced vasoconstriction, since the complex III inhibitor antimycin A also attenuates vasoconstriction elicited by the thromboxane analogue U46619 under conditions of blocked NO synthesis in the isolated perfused rabbit lung . In our model, murine intra-acinar arteries responded to antimycin A with a reversal of HPV to vasodilation although U46619-induced constriction was unimpaired, arguing for a critical role of complex III in HPV of this vascular segment.
The present data provide also evidence for an additional role of complex II in intra-acinar HPV. Complex II is a component of both the Krebs cycle, here also termed succinate dehydrogenase (SDH), and the mitochondrial electron transport chain. It consists of two integral proteins of the inner mitochondrial membrane (SDH-C, SDH-D) that together comprise the heme protein cytochrome b560, and two peripheral parts exposed to the mitochondrial matrix, SDH-A and SDH-B [39, 40]. The catalytic centre for the enzymatic conversion of succinate to fumarate is located at the flavoprotein SDH-A, and electrons flow along iron-sulphur clusters of SDH-B towards SDH-C/D to, finally, reduce ubiquinon to ubiquinol. There are conditions, however, under which electrons flow in reverse direction so that this complex acts, then, as fumarate reductase . This has been directly shown for isolated mitochondria of the bovine heart and for the rat heart in anoxia or severe hypoxia [41, 42]. We have recently obtained evidence for catalytic switch of SDH to fumarate reductase in the course of cellular adaptations to hypoxia in rat sensory neurons and small mouse pulmonary vessels [18, 43]. An SDH mutation causes oxidative stress in nematodes , and in Escherichia coli, where succinate oxidation and fumarate reduction are accomplished by two structurally different enzymes, fumarate reductase is an extremely efficient generator of ROS . Accordingly, complex II activity is essential for hypoxia-induced ROS generation in the pulmonary vasculature .
Hence, we have put forward the hypothesis that catalytic switch of complex II to fumarate reductase with concomitant enhanced ROS generation is part of the hypoxia-sensor and -signalling mechanisms in the pulmonary vasculature. Consistent with this concept, succinate, but not fumarate, prevented development of intra-acinar HPV in our present PCLS experiments, which can be explained if complex II acts as fumarate reductase and is inhibited by excess of its reaction product, succinate. It has to be taken into account, however, that succinate and fumarate also exert additional effects. For instance, succinate inhibits prolyl hydroxylases that, in an oxygen-dependent manner, regulate the stability of hypoxia-inducible transcription factor , and succinate can also interfere with neurotransmitter receptors . Blockade of HPV by the irreversible inhibitor of the enzymatic centre of SDH-A, 3-NPA, supported the notion of requirement of active complex II for intra-acinar hypoxic constriction. Similarly, inhibition of HPV was achieved by the general flavoprotein inhibitor DPI which also acts upon SDH-A. On the other hand, TTFA, inhibiting complex II by occupying its ubiquinone binding sites , was not fully effective in preventing intra-acinar HPV. It has to be taken into account, however, that TTFA also targets extra-mitochondrial enzymes such as esterases  so that partly counteracting effects might have been triggered.
Within the respiratory chain, ROS are generated upstream of complex IV at either of the complexes I-III. Thus, the assumption of an involvement of ROS generation in HPV is consistent with the view that HPV is triggered by events located upstream of complex IV. Accordingly, this complex is generally not considered as being specifically involved with HPV, although an unusual cytochrome a3 residing in complex IV has been associated with acute oxygen sensing in the carotid body [50, 51] and a recent study also suggests its participation in sustained HPV . In our present experiments, the complex IV inhibitor, NaN3, abrogated HPV and also largely reduced U46619-induced constriction. These data argue for an unspecific impairment of intra-acinar vasoconstriction by NaN3 rather than for a specific participation of complex IV in HPV. In line with these data, we have recently shown that NaN3 also does not block hypoxia-induced ROS generation in smallest intrapulmonary vessels in the mouse .
This study establishes the first model for studying basic characteristics of HPV directly in intra-acinar murine pulmonary vessels, demonstrating a monophasic constrictory response that starts to fade after 40 min. Collectively, the data obtained by various respiratory chain inhibitors and metabolites provide evidence for a critical involvement of the generation of ROS and of mitochondrial complexes II and III in intra-acinar HPV. A general drawback of studies involving classical inhibitors and metabolites, however, is their limited specificity. Since the present model is based upon murine PCLS kept in short-term slice cultures, it provides a promising tool to overcome these problems in future studies by use of genetically engineered mouse strains and siRNA application in vitro.
The authors thank Marco Gruß for help in the measurement of pO2 of the medium. The financial support of the Deutsche Forschungsgemeinschaft (Sonderforschungsbereich 547, project C1) is gratefully acknowledged.
- 6.Grimminger F, Weissmann N, Spriestersbach R, Becker E, Rosseau S, Seeger W: Effects of NADPH oxidase inhibitors on hypoxic vasoconstriction in buffer-perfused rabbit lungs. Am J Physiol 1995, 268:747–752.Google Scholar
- 9.De Mello D, Reid LM: Arteries and veins. In The Lung: Scientific Foundations. Volume 1. Edited by: Crystal RG, West JB. New York:Raven Press; 1991:767–778.Google Scholar
- 11.Porcelli RJ: Pulmonary Hemodynamics. In Treatise on Pulmonary Pharmacology. Comparative Biology of the Normal Lung. Volume 1. Edited by: Parent RA. Boca Raton: CRC Press; 1991:241–270.Google Scholar
- 23.Speyer CL, Steffes CP, Tyburski JG, Ram JL: Lipopolysaccharide induces relaxation in lung pericytes by an iNOS-independent mechanism. Am J Physiol Lung Cell Mol Physiol 2000, 278:880–887.Google Scholar
- 24.Williams M, Kerkar S, Tyburski JG, Steffes CP, Carlin AM, Wilson RF: The roles of cyclic adenosine monophosphate- and cyclic guanosine monophosphate-dependent protein kinase pathways in hydrogen peroxide-induced contractility of microvascular lung pericytes. J Trauma 2003, 55:677–682.CrossRefPubMedGoogle Scholar
- 28.Weissmann N, Manz D, Buchspies D, Keller S, Mehling T, Voswinckel R, Quanz K, Ghofrani HA, Schermuly RT, Fink L, Seeger W, Gassmann M, Grimminger F: Congenital erythropoietin over-expression causes "anti-pulmonary hypertensive" structural and functional changes in mice, both in normoxia and hypoxia. Thromb Haemost 2005, 94:630–638.PubMedGoogle Scholar
- 36.Monaco JA, Burke-Wolin T: NO and H 2 O 2 mechanisms of guanylate cyclase activation in oxygen-dependent responses of rat pulmonary circulation. Am J Physiol 1995, 268:546–550.Google Scholar
- 37.Weissmann N, Grimminger F, Voswinckel R, Conzen J, Seeger W: Nitro blue tetrazolium inhibits but does not mimic hypoxic vasoconstriction in isolated rabbit lungs. Am J Physiol 1998, 274:721–727.Google Scholar
- 47.Roehrs C, Garrido-Sanabria ER, Da Silva AC, Faria LC, Sinhorin VD, Marques RH, Priel MR, Rubin MA, Cavalheiro EA, Mello CF: Succinate increases neuronal post-synaptic excitatory potentials in vitro and induces convulsive behavior through N-methyl-d-aspartate-mediated mechanisms. Neuroscience 2004, 125:965–71.CrossRefPubMedGoogle Scholar
This article is published under license to BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.