A qualitative and quantitative study of the lung of an ostrich, Struthio camelus
Department of Anatomical Sciences, The University of the Witwatersrand, 7 York Road, Parktown, Johannesburg 2193, South Africa
*e-mail: 055john{at}chiron.wits.ac.za
Accepted April 24, 2001
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Summary |
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Key words: ostrich, Struthio camelus, lung, ratite, birds, respiration, size, morphology, morphometry.
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Introduction |
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Among birds, the colossal body size, the relinquishment of volancy and survival in an exacting habitat should have imposed certain constraints and prescribed particular physiological and morphological novelties on the biology of the ostrich. Compared with the smaller volant birds that can utilize adiabatic cooling and convective heat loss at altitude, the ostrich has to tolerate extreme thermal stresses on the ground. This is exacerbated by the fact that it is too large to seek cover and protection easily in more hospitable microclimates that may chance in its ecosystem. The intense selective pressure that the ostrich has endured in the past is clearly demonstrated by the now very restricted distribution of a once very extensive natural geographical distribution. Animals that live in extreme environments (e.g. Schmidt-Nielsen, 1964; Dawson and Schmidt-Nielsen, 1964; King and Farner, 1964) and those that face intense selective pressures must inescapably evolve certain adaptations or face extinction. Such features have been reported in the ostrich (e.g. Louw et al., 1969).
The physiology of the ratites, a taxon phylogenetically considered to fall among the most primitive of the extant birds (e.g. Storer, 1971a; Storer, 1971b), differs from that of other birds in certain fundamental ways. While other birds have a body temperature ranging from 4042°C (e.g. Irving and Krog, 1954; McNab, 1966), the large flightless birds generally have a lower body temperature that ranges from 38.139.7°C (King and Farner, 1961; Bligh and Hartley, 1965; Crawford and Schmidt-Nielsen, 1967; Crawford and Lasiewski, 1968; Louw et al., 1969; Calder and Dawson, 1978; Jones et al., 1983). Of the seven species of birds studied by Lutz et al. (Lutz et al., 1974), the rhea Rhea americana had the highest oxygen affinity of blood (P50=2.8kPa). While Calder and Schmidt-Nielsen (Calder and Schmidt-Nielsen, 1966; Calder and Schmidt-Nielsen, 1968) demonstrated that many species of panting birds show extreme hyperventilatory hypocapnia and alkalosis after several hours of exposure to thermal stress, the ostrich and the emu, Dromiceius novaehollandiae, maintain resting values of arterial PCO2 (PaCO2) and pH while panting continuously for as long a 6h under high (56°C) ambient temperature (Schmidt-Nielsen et al., 1969; Jones, 1982a; Jones et al., 1983). Studies that have alluded to the existence of a similar acidbase stabilizing peculiarity with thermal panting in nonratite birds (e.g. Calder and Schmidt-Nielsen, 1966; Calder and Schmidt-Nielsen, 1968; Bouverot et al., 1974; Marder et al., 1974; Marder and Arad, 1975; Ramirez and Bernstein, 1976; Krauzs et al., 1977) are somewhat equivocal owing to certain important departures in the experimental procedures applied compared with those used on the ostrich (Schmidt-Nielsen et al., 1969; Jones, 1982a) and the emu (Jones et al., 1983).
Although the anatomy of the air sacs has been studied (Macalister, 1864; Roché, 1888; Schulze, 1908; Bezuidenhout, 1981; Bezuidenhout et al., 1999), morphological and morphometric studies on the ostrich lung, which should greatly help explain the exceptional respiratory physiology of the bird, are lacking. The goal of this study was to outline, both qualitatively and quantitatively, the structure of the ostrich lung to attempt to answer the following fundamental question: how does the design of the ostrich lung explain the unique physiological processes by which the bird attains a remarkable exercise capacity and toleration of the most severe heat loads of any bird by sustained panting while maintaining PaCO2 at near resting values, i.e. without experiencing acidbase imbalance of the blood? It is hoped that the details given here may help to explain or may be used to resolve the unsettled questions on the physiology of the avian respiratory system and that of the ostrich in particular.
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Materials and methods |
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The ostrich was killed by intravenous injection with 15ml of Euthanase (200mg cm3 sodium barbitone) into the brachial vein. A ventral midline incision was made along the neck and the larynx, and the trachea was exteriorized and cannulated. Stock solution (3l) of Cumplucad anatomic solution (CAS) (International Zaragoza, Spain; osmolarity, 360mosmoll-1) was instilled down the trachea from a height of 30 cm above the highest point (the sternum) of the supine bird (CAS is a recently marketed organic peroxide- and alcohol-based fixative). The trachea was ligated below the cannula, and the fixative was left in the lungs. After 3h, the sternum was removed to expose the lungs and some of the unavoidably damaged air sacs. The angle of bifurcation of the trachea into the extrapulmonary primary bronchi (EPPB) was determined while the lungs were still in situ, i.e. in their anatomical positions. Together with the attached trachea, the lungs were carefully dissected out from the deep costal insertions and immersed in fresh fixative. They were closely examined and found to be free of disease and physical damage. The lengths and diameters of the trachea, the EPPB, the intrapulmonary primary bronchi (IPPB), i.e. the mesobronchi, as well as the angles between the IPPB and the medioventral secondary bronchi (MVSB), were determined. The angles and diameters of the MVSB were measured after the lung had been isolated from the EPPB, dissected and a cast impression made using dental plastic (Pratley).
Determination of the volume of the lung
The connective tissue and fat adherent to the lung were trimmed off. The large ostium opening into the caudal thoracic and abdominal air sacs and the opening to the EPPB (at the hilus) were plugged tightly with plastic paper (to avoid entry of water into the lung), and the volumes of the left and right lungs were individually determined by the water displacement method. A lung was slowly immersed into a container completely filled with water, the displaced water was collected in an outer container and the volume measured. Estimations were repeated, each time after mopping the lung dry, until three consistent values were obtained. The mean of such readings was taken to be the volume of the lung. The right lung was used for morphometric analysis and the left for morphological study.
Sampling and morphometric analyses of the lung
Three dorsoventral cuts were made along the last three most prominent costal sulci of the right lung, giving four parts; the first sulcus was avoided because it was relatively more superficial, and a slice made along it would not pass through the primary bronchus owing to the caudomedial location of the hilus. The avian lung being reasonably homogeneous, especially at the parabronchial and parenchymal levels (e.g. Maina, 1988), the sulci were taken as predetermined (unbiased) sampling landmarks from which complete cross sections of the lung were taken craniocaudally (rather like stratified serial sections) for both light and transmission electron microscopic analyses.
A quadratic lattice grid was laid on the cranial face of each slice, and the volume densities (VV) of the exchange tissue (VVet), the lumina of the secondary bronchi and parabronchi (tertiary bronchi) (VVsp), the large blood vessels (<0.5 mm diameter) (VVlb) and the primary bronchus (VVpb) were determined: this constituted the first level (gross) of the four strata of the morphometric analyses (see Table1). With the cranial face uppermost, the slices were laid out flat and cut into dorsal and ventral parts immediately dorsal to the IPPB. This gave rise to a total of eight half-slices that were lettered from A to H. Along their craniocaudal thicknesses, the half-slices were subsequently cut into halves: these are referred to as half-half-slices.
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Light microscopy
Tissue samples for light microscopy were processed by standard laboratory techniques and embedded in paraffin wax. Sections were cut at a thickness of 10µm, stretched out on a hot water bath (40°C), mounted on glass slides and stained with Haematoxylin and Eosin. Comparison of the dimensions of the mounted and stained sections with the size of the tissue block face was used to check for compression of the sections. From each tissue sample, the first technically adequate, i.e. non-compressed, well-stained section was used for morphometric analysis. The volume densities of the exchange tissue (VVet), the lumina of the parabronchi (VVpl), the blood vessels between 20µm and 0.5 mm in diameter (VVsv) were determined by point-counting using an ocular Zeiss integrating graticule with an etched quadratic lattice grid at a magnification of x100: the analysis was carried out field by field until the entire section had been covered: this constituted the second level of the morphometric analyses (see Table1). To determine the adequacy of the sections analysed, a summation average graph was plotted, and the points counted were checked against a standard nomogram given by Weibel (Weibel, 1979, p. 114). Except for the primary bronchus, which constituted a relatively small fraction of the lung, the number of points counted for each of the structural components gave a standard error of less than 2%.
Transmission electron microscopy
Since the effectiveness and permanence of CAS in fixing tissues for transmission electron microscopy was uncertain, the sampled pieces were refixed in 2.3% glutaraldehyde buffered in sodium cacodylate (osmolarity 360mosmoll-1; pH7.4 at 23°C) for 6h. Subsequently, for 3h, the tissue samples were post-fixed in 1% osmium tetroxide buffered in 1moll-1 sodium cacodylate (pH7.4 at 23°C; total osmolarity 350mosmoll-1). This was followed by block staining with 0.5% uranyl acetate buffered with 0.05moll-1 sodium hydride maleate adjusted by sodium hydroxide (pH4.8 at 23°C; total osmolarity 100mosmoll-1). The tissues were dehydrated in a graded series of ethanol concentrations from 70% to absolute and two changes in acetone, then infiltrated and embedded in epoxy resin (Epon 812).
Blocks were prepared from pieces derived from different areas of a half-half-slice, a block was picked at random, and semithin sections were cut and stained with Toluidene Blue. The sections were viewed on a Kontron Image Analyzer (Zeiss Instruments) at a magnification of x3200 with a superimposed quadratic lattice grid: this constituted the third level of the hierarchical morphometric analyses (Table1). The volume densities of the components of the exchange tissue, i.e. the air capillaries (VVac), blood capillaries (VVbc) and supporting tissue [i.e. the tissue involved in gas exchange (tissue of the bloodgas barrier, VVbg), and the tissue not involved in gas exchange, VVte (i.e. where blood or air capillaries directly connect; see Fig.10)] were determined by point-counting. The surface densities (SV) of the air capillaries (SVac), bloodgas (tissue) barrier (SVbg), capillary endothelium (SVce), erythrocytes (SVer) and tissue not involved in gas exchange (SVte) were determined by intersection-counting (Weibel, 1979). The absolute volumes and the surface areas were calculated from the volumes of the lung and that of the exchange tissue (Vet), as appropriate. The surface area of the plasma layer was estimated as the mean of that of the capillary endothelium and the erythrocytes and the surface density of the bloodgas tissue barrier as the ratio of its surface area to Vet.
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Computer-generated three-dimensional structural model
On the basis of the actual dimensions and geometries of the trachea, EPPP, IPPB and MVSB, a three-dimensional model of the conduits that are directly involved in inspiratory aerodynamic valving (IAV), a process through which the inspired air is shunted across the openings of the MVSB (e.g. Banzett et al., 1987; Butler et al., 1988; Wang et al., 1992) was drawn in CFX 5.4, a computational fluid dynamics (CFD) program. Compared with certain other birds (Maina and Africa, 2000), the ostrich lacks a segmentum accelerans (SA) at the terminal part of the EPPB. Conceivably, in the ostrich, the exceptionally large sizes and the particular geometry of the bronchial system in an exceptionally large bird may explain IAV: the airflow dynamics in the airways of the lung may differ significantly from those in the smaller birds. CFD is a computer-based tool for simulating the behaviour of systems involving fluid flow, heat transfer and other related physical processes. The technical and mathematical details entailed in the plotting, simulation of the airflow and interpretation of the results will be reported in a subsequent paper. Here, reconstructed three-dimensional views of the geometry and the relative sizes of the air-conduits involved in IAV (see Fig.11) are given to help the reader sufficiently to conceptualize the morphological descriptions. Certain deviations from the actual geometry were inevitable because of software limitations and the complexity of the airway system itself. Furthermore, the diameters and the lengths of all the airtubes are shown as fixed, implying a rigid structure. This may not be the case in life.
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Results |
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Discussion |
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The conspicuous dearth of morphological and morphometric data on the ostrich lung can be attributed to various reasons: (i) the logistical difficulties of obtaining live healthy specimens from which fresh lung tissues can be adequately fixed for meaningful microscopy (in South Africa, in particular, although not strictly threatened, wild ostriches are protected and the extremely competitive and lucrative nature of commercial ostrich production presently constrains the availability of live specimens, especially for terminal experiments), (ii) problems with handling and restraining a large, highly irritable and dangerous bird and, (iii) inexplicable technical problems and uncertainties in fixing the lung for microscopic studies. The ostrich lung is characteristic of the avian lung, being connected to capacious air sacs, some of which extend out of the coelomic cavity into the surrounding anatomical spaces and structures such as bones and even the skin (e.g. Bezuidenhout et al., 1999). Intratracheal instillation is technically the most direct method used for fixing lungs for microscopic morphometry and modelling: it preserves the vascular elements (particularly the erythrocytes) that are important elements in characterizing a lungs structural competence for gas exchange (e.g. Weibel, 1984; Bur et al., 1985). Furthermore, intravascular perfusion has been reported to cause a relatively greater degree of shrinkage than intratracheal instillation (e.g. Gil et al., 1979; Bachofen et al., 1982; Crapo et al., 1988). In birds in general and in the ostrich in particular, because of its exceptional size, fixing the lung by pouring the fixative down the trachea is like attempting to fill a large, highly perforated container with water. Since, according to physical laws, a fluid follows the line of least resistance, in such a design the fixative only reaches the lung if and when the air sacs and their extensive diverticulae (conceptually an external-limiting container) are filled up with fixative. At this point, the pressure build-up forces the fixative into the lung and subsequently into the very narrow terminal gas-exchange units, the air capillaries. Since the very nature of the lung is highly perforate, the fixation of the avian lung must be performed in situ, so even when the fixative stops flowing down the trachea (suggesting that the lung and the air sacs are filled up with fixative) there is no absolute certainty that the fixative has reached the most distant parts of the pulmonary airway system.
Our earlier attempts to fix the lungs of as many as six wild ostrich specimens in the field by intratracheal instillation with 2.3% glutaraldehyde buffered with sodium cacodylate, a method that has been used with remarkable success on relatively smaller species of birds for microscopic morphometry (e.g. Dubach, 1981; Abdalla et al., 1982; Maina, 1982; Maina et al., 1989), was in all cases unsatisfactory. It would appear that, inexplicably, controlled laboratory conditions and the use of particular fixatives are important for the successful fixation of the ostrich lung. In the present study, we used CAS, a newly marketed fixative that offers particular advantage over conventional aldehyde-based fixatives in that it is not irritating to the eye and respiratory passages, causes minimal tissue shrinkage and maintains the tissue consistency almost in the in vivo state. Considering that only 3l of CAS was used to fix a large perforated lung and much of the fixative flowed down the trachea, IPPB and ostia into the capacious air sacs (a process confirmed after the coelomic cavity was opened), we envisage that the peroxide and alcohol vapours penetrated and fixed the lung tissue. Fixation of the mammalian lung using formalin vapour was first performed by Weibel and Vidone (Weibel and Vidone, 1962) and Weibel (Weibel, 1963), and subsequently by Dunnill (Dunnill, 1968). Using vapourized fixative on lungs is a judicious approach since it emulates the salient natural state that prevails during life, where the organ is filled with a gas (air), not a liquid. Owing to their much greater densities, liquid-based fixatives may cause changes in the size of the airways and location of the vascular elements of the lung. Unfortunately, many gaseous fixatives, including vapourized formalin (e.g. Weibel, 1970/71), do not confer satisfactory preservation of tissues especially to the high level required for electron microscopy. Use of CAS, at least followed by 2.3% glutaraldehyde buffered in sodium cacodylate, appears to offer satisfactory fixation for transmission electron microscopy (see Fig.10).
The osmolarity of the fully constituted fixative is a critical factor in a morphometric analysis. A hyperosmotic fixative will cause tissue shrinkage, while a hypo-osmotic one may lead to tissue swelling and histological and ultrastructural imperfections. The degree of shrinkage caused by various fixatives and the contributions that buffers and fixatives themselves make to the overall osmolarity of a constituted fixative has long been debated (e.g. Weibel, 1963; Hayat, 1970; Eisenberg and Mobley, 1975; Barnard, 1976; Mathieu et al., 1978; Weibel, 1979; Lee et al., 1980; Mazzone et al., 1980; Wangensteen et al., 1981; Bastacky et al., 1985; Gehr and Crapo, 1988), and the issue is far from resolved. As a guiding principle, the fixative, buffer and other reagents used in processing biological tissues for microscopy should be chosen to maintain the qualitative and quantitative attributes of the tissues as close to their in vivo state as possible. Where necessary, shrinkage constants should be determined and, if significant, used to adjust the measurements. The osmolarity of CAS, the primary fixative used in the present, was 365mosmoll-1 while that of the secondary fixative, i.e. 2.3% glutaraldehyde buffered in sodium cacodylate, was 350mosmoll-1. These values are reasonably close to the osmolarity of 340mosmoll-1 determined for the blood plasma of the domestic fowl Gallus gallus var. domesticus (Sykes, 1971). Assuming that the osmolarity of the blood plasma in the ostrich is similar to that of the chicken, the use of approximately equiosmolar fixatives should have caused minimal shrinkage of the ostrich lung tissue.
The morphological features that were observed and the morphometric values that were determined in the ostrich lung suggest that this bird is particularly well adapted for gas exchange. The absence of the interparabronchial septa (IPS) indicates that the lung of the specimen examined in this study, which based on its body mass, would be considered to be juvenile, was fully developed. As can be inferred from earlier studies (e.g. Juillet, 1912; Locy and Larsell, 1916; Jones and Radnor, 1972), during the early stages of the development of the avian lung, the parabronchi (tertiary bronchi) are generally separated by septal connective tissue, giving them a somewhat hexagonal shape. In some species, the IPS persist throughout life, while in others, often the highly derived more energetic species (e.g. Duncker, 1972; Duncker, 1974; Duncker, 1979; Dubach, 1981; Maina et al., 1982), they are lost at various stages of development; when present, the IPS support the parabronchial blood vessels. Early maturity of the pulmonary system, as appears to occur in the ostrich, would be an adaptive feature in an energetic bird exposed to intense predation. The lung of the emu, the only extant member of the family Dromaiidae and the most widespread of the Australian flightless birds (e.g. Cameron and Harrison, 1978), lacks IPS (Maina and King, 1989). Potentially, the rhea has a high aerobic capacity (Bundle et al., 1999), but no morphological investigation has been carried on its lung. In the ostrich, the very shallow atria that line the parabronchial lumina should minimize the diffusional distance of oxygen to the air capillaries, enhancing the gas-exchange efficiency. Unlike the species of birds that have so far been investigated (e.g. Maina, 1982; Maina, 1989; Maina et al., 1989), a conspicuous difference between the volumes of the right and the left lungs was observed in the ostrich: the volume of the left lung was 9% greater than that of the right lung. Furthermore, conspicuous diameter, length and geometrical differences between the right and left EPPB were observed: the right EPPB was longer, narrower and more horizontal, while the left EPPB was shorter, wider and more vertical. The pulmonary and bronchial morphological differences that occurred in the ostrich were similar to those found in the human, but interestingly in the opposite pattern: in the human respiratory system, the right lung is larger than the left and the right primary bronchus is shorter, wider and more vertical (e.g. Romanes, 1972). Jones (Jones, 1982a) observed no significant difference in the lung mass between the left and the right lungs of the ostrich in the blood flow to the two lungs during resting and panting. Although Schulze (Schulze, 1908) described four groups of MVSB (his bronchi ventrales) in the ostrich, we could only find three MVSB, even after the preparation of plastic impressions that greatly improved the visualization of the dissected airways. It is difficult to establish the authenticity of Schulzes (Schulze, 1908) observations since his account completely lacks illustrations of pulmonary morphology. It was, however, quite evident in the present study that the number of MVSB in the ostrich lung could be mistaken, particularly because the large first MVSB bifurcates close to the primary bronchus (see Fig.3, Fig.5). The majority of birds have four MVSB (e.g. McLelland, 1989), some have five (e.g. cassowaries; Dotterweich, 1930) or even six (e.g. pelicans; e.g. Schulze, 1910). The developmental and functional significance of these differences is unclear.
Although wide-ranging extrapolations based on data from a single specimen may not be justifiable, among birds (e.g. Dubach, 1981; Maina et al., 1982; Maina, 1989; Maina et al., 1989), the ostrich lung has the highest volume density of the exchange tissue (VVet) of 78.31% (Table2). Clearly, the high VVet has formed at the expense of the lumina of the parabronchi, the secondary bronchi and the large blood vessels (Table2). The large unventilated volume of the exchange tissue during protracted thermal panting may conceivably offer a substantial reservoir of carbon dioxide, presumably explaining the absence of respiratory alkalosis during such stressful conditions. Compared with the seven species of birds selected for comparison in Table2, Table3, Table4 and Table5 (for a comprehensive summary of the pulmonary morphometric data available on the avian lung, see Maina, 1982; Maina, 1989; Maina et al., 1989), the mass-specific lung volume of the ostrich (VLM-1; 39.1 cm3kg-1) was exceeded only by that of the hummingbird Colibri coruscans (Table4). The ht of the ostrich lung was remarkably high (0.56µm) (Table5), comparable with that reported in the Humboldti penguin Sphenicus humboldti (0.53µm) (Maina and King, 1987). The thick bloodgas (tissue) barrier in the penguin was attributed to a need to secure mechanical and functional integrity of the lung under high hydrodynamic pressure during dives (Welsch and Aschauer, 1986). While the ostrich is not subjected to same conditions, in a bird that may reach a height of 3m, the lung may experience considerable hypostatic congestion. This may necessitate the development of a thick tissue barrier to ensure physical fitness. Moreover, during high-speed running, when large volumes of blood pass through the lung, a thick tissue barrier may help to avoid damage to the pulmonary vasculature. Although measurements are lacking in the ostrich itself, systemic blood pressures in birds in general are remarkably high. Speckman and Ringer (Speckman and Ringer, 1963) determined a systolic blood pressure of 53kPa in a resting domestic turkey Melleagris gallopavo. As commonly observed at post mortem, especially in domestic species of birds in which the functional capacities have been compromised through intense genetic breeding for properties, such as rapid weight gain and egg production (e.g. Smith, 1985; Gyles, 1989; Ross Breeders, 1999), sudden deaths in birds occasionally associated with fright result from arterial rupture (e.g. Carlson, 1960; Hamlin and Kondrich, 1969). Although the tissue barrier in the ostrich was remarkably thick compared with that of other birds (e.g. Maina, 1989; Maina et al., 1989), the plasma layer in the ostrich lung was remarkably thin (0.14µm; Table1). Compensatory adaptive structural strategies in the components of the airhaemoglobin pathway are a common feature of the design of the avian lung. In the penguin Spheniscus humboldti, e.g. while the tissue barrier was thick, DLO2 was greatly enhanced by a large Vc.
The mass-specific surface area of the tissue barrier (StM-1) (Table4) was relatively high in the ostrich (30.1 cm2g-1) compared with that of non-flying birds such as the emu (5.4 cm2g-1) (Maina and King, 1989), the penguin (18.1 cm2g-1) (Maina and King, 1987) and the domestic fowl (8.7 cm2g-1) (Abdalla et al., 1982). In the ostrich, an extensive respiratory surface area has offset a thick tissue barrier, giving a DtO2M-1 of 0.0022mlO2s-1Pa-1kg-1, the highest value in the two non-flying avian taxa (emu and penguin) selected for comparison (Table5). The VcM-1 in the ostrich lung (6.25 cm3kg-1) was only exceeded by that of the penguin Spheniscus humboldti (8.0 cm3kg-1) (Table5). Diving animals have high mass-specific blood volumes (e.g. Lenfant et al., 1970; Stephenson et al., 1988; Butler, 1991a), much of it being found in the lungs. The VcM-1 in the ostrich was comparable with that of small volant birds such as the hummingbird Colibri coruscans (6.57 cm3kg-1) and the house sparrow (6.4 cm3kg-1). A large VcM-1 enhanced the DLO2M-1 giving a mass-specific value of 0.00073mlO2s-1Pa-1kg-1 (Table5): this value was only exceeded by that of the house sparrow (0.00093mlO2s-1Pa-1kg-1). Unfortunately, this variable was not determined by Dubach (Dubach, 1981) for the humming bird. The capillary loading, i.e. the ratio of the pulmonary capillary blood volume (Vc) to the respiratory surface area (St), indicates the degree of exposure of blood to air. In the ostrich, VcSt-1 was 2.08 cm3m-2, interestingly a value that was lower than that of the emu (9.5 cm3m-2) and the penguin (4.4 cm3m-2) (Table5): the low VcSt-1 in the ostrich is highly favourable for gas exchange since pulmonary capillary blood (Vc) is exposed to air over an extensive respiratory surface area. The substantial pulmonary morphometric differences between the ostrich and the emu may be explained by the fact that the latter lives in an environment that has relatively fewer predators.
Although the ostrich is flightless, it is an exceptionally energetic bird. It can achieve and sustain speeds as high as 90 kmh-1, making it the fastest ground-running bird (e.g. Cameron and Harrison, 1978; Fisher and Peterson, 1988). All the extant flightless birds have evolved secondarily from volant ancestors (e.g. Fisher and Peterson, 1988; Pough et al., 1989). Interestingly, they appear to have conserved the cardiopulmonary fitness of the latter (e.g. Brackenbury, 1991; Bundle et al., 1999). While considerable variation occurs among species, birds can increase their metabolic rates by factors ranging from 8 to 15 between rest and exercise (e.g. Lasiewski, 1963; LeFebvre, 1964; Tucker, 1968; Tucker, 1972; Torre-Bueno, 1985; Brackenbury and Avery, 1980; Grubb et al., 1983; Butler, 1991b). Birds trained to run on a treadmill can achieve maximum metabolic rates that approach those measured during flight (Brackenbury, 1991) and that far exceed those of terrestrial mammals under same conditions (e.g. Bundle et al., 1999). The relative metabolic capabilities of flying, running and swimming birds appear to be limited not directly by oxygen delivery but rather by the relative masses and aerobic capacities of the working muscles (e.g. Turner and Butler, 1988; Brackenbury, 1991). Bipedal runners such as the ratite birds use more energy for a given rate of force production because they require a greater mass of muscle to support their body weight (Roberts et al., 1998): on average, birds use 1.7 times more metabolic energy than the quadrupeds. In the rhea, the locomotory muscles constitute approximately 30% of the body mass (Bundle et al., 1999). Energy constraints for locomotion may partly explain why the ostrich (the largest extant bird) is over 30 times smaller than the elephant (the largest extant land mammal). The mass-specific resting rate of oxygen consumption (V·O2M-1) of the ostrich is 4.72mlO2min-1kg-1 (Schmidt-Nielsen et al., 1969) compared with 3.91mlO2min-1kg-1 (Crawford and Lasiewski, 1968) or 4.2mlO2min-1kg-1 (Grubb et al., 1983) for the emu, and 5.28mlO2min-1kg-1 (Crawford and Lasiewski, 1968) for the rhea. The emu can increase its V·O2 approximately 11.4 times above resting (Grubb et al., 1983). Within 2min of termination of an 11km run at a speed of 17kmh-1, the V·O2M-1 of the ostrich was 31.35mlO2min-1kg-1 (Schmidt-Nielsen et al., 1969), giving a factorial increase of V·O2 from rest to exercise of approximately 7. King and Farner (1961) pointed out that the V·O2 of the ostrich was approximately 30% higher than that predictable from its body size. This was, however, disputed by Crawford and Schmidt-Nielsen (Crawford and Schmidt-Nielsen, 1967). In the rhea, Bundle et al. (Bundle et al., 1999) observed that, while running on an inclined treadmill, the upper limit of aerobic metabolism was 36 times the minimum resting rate, a factorial increase exceeding that reported for nearly all mammals: a V·O2max of 171mlO2min-1kg-1 was reached at a speed of 14.4kmh-1.
Since the ostrich and the emu can pant for a long time without undergoing respiratory alkalosis (Schmidt-Nielsen et al., 1969; Jones, 1982a; Jones, 1982b; Jones et al., 1983), an efficient expiratory aerodynamic valving (EAV) mechanism must operate in their respiratory systems. During resting breathing, the expired air is directed into the gas-exchange tissue of the paleopulmo through the openings of the MDSB. During thermal panting, the increased airflow from the caudal air sacs is directed into the IPPB onwards to the trachea. The hypoxaemic state that befalls a panting ostrich (Schmidt-Nielsen et al., 1969; Jones, 1982a; Jones, 1982b) or emu (Jones et al., 1983) may result from a combination of several factors, e.g. partitioning of pulmonary blood flow and/or shifts in the airflow pathways. Jones (Jones, 1982a) observed significant changes in the blood flow patterns between the paleopulmic and the neopulmonic regions of the ostrich lung when it changed from resting to panting. In other birds, however, the expired air is invariably directed into the MDSB (e.g. Brown et al., 1995) and then into the gas-exchange tissue regardless of the respiratory state. In the non-ratite birds, switching of the expiratory outflow pathways may be lacking or the process may be imperceptably less effective. The hyperventilatory airflow through the exchange tissue during thermal panting makes the nonratite birds hypocapnic and alkalotic (e.g. Bouverot et al., 1974; Marder et al., 1974; Marder and Arad, 1975; Ramirez and Bernstein, 1976; Krauzs et al., 1977). Compared with other birds, the ratite birds experience thermal stress under different conditions and circumstances: heat stress usually occurs when the birds are resting on the ground, a state in which the V·O2 is low. In the volant birds, however, the greatest need for heat dissipation occurs during exercise (flight), when V·O2 is high. While the ratites can afford to disengage the two processes (i.e. gas exchange and heat dissipation) this is impracticable in flying birds. Such functional conflicts suggest underlying morphological differences in the respiratory designs of the ratite and nonratite groups of birds. The ostrich has very well-developed capacious air sacs (Schmidt-Nielsen et al., 1969; Bezuidenhout et al., 1999): the volume of air sacs in a 100kg ostrich is approximately 15l, the caudal thoracic air sac being the largest (Schmidt-Nielsen et al., 1969). Boggs et al. (Boggs et al., 1998) suggested that locomotion in swimming birds might isochronally compress the caudal air sacs more than the cranial ones, forcing air through the lung: such a process may also enhance gas exchange in a running ostrich. Correlation between locomotion and respiration has been reported in other groups of animals such as lizards (e.g. Carrier, 1991) and bats (e.g. Thomas, 1987). The ostrich can maintain its body temperature below 40°C even when exposed to ambient temperatures of 56°C for more than 6h (Schmidt-Nielsen et al., 1969). Crawford and Schmidt-Nielsen (Crawford and Schmidt-Nielsen, 1967) suggested that, during thermal stress, the air sacs provide evaporative cooling as the gas-exchange surfaces of the lungs are bypassed, while Bert (Bert, 1870) pointed out that the very survival of the ostrich in the Sahara was made possible by the role of the air sacs in cooling the body.
Morphological features of physiological significance were observed in the lung of the ostrich. The neopulmo is very poorly developed, consisting of a few laterodorsal secondary bronchi that arise from the most caudal part of the primary bronchus, their laterally directed parabronchi and the connections of the parabronchi with the caudal thoracic and abdominal air sacs. The MDSB are superficially located, making them easily accessible for sampling respiratory gases and experimental investigations of processes such as airflow dynamics. The ostrich lung conspicuously lacks a segmentum accelerans (SA), an epithelial tumescence at the terminal part of the EPPB (Maina and Africa, 2000). Wang et al. (Wang et al., 1992) associated the SA with inspiratory aerodynamic valving, i.e. the shunting of air past the openings of the MVSB. An SA was observed in the lung of the flightless domestic fowl (Maina and Africa, 2000) and may be of greater phylogenetic than functional significance. However, the domestic fowl has been domesticated from the wild jungle fowl Gallus gallus of South-East Asia for only the last 8000 years approximately (e.g. West and Zhou, 1988), which in evolutionary terms may not have been long enough for the loss of morphological features that may have been requisite for volancy. It is conceivable that, during thermal panting, the presence of an SA at the terminal part of the EPPB could impede the flow of the expired air from the IPPB to the trachea, deflecting some of it into the MVSB and subsequently into the cranial air sacs. Theoretically, this would create a nonrespiratory loop that would compromise both thermoregulation and gas exchange. The SA appears to be more important for shunting inspired air past the openings of the MVSB during resting (e.g. Banzett et al., 1987; Banzett et al., 1991; Wang et al., 1992). These investigators speculated that as a means of reducing the energetic cost of breathing, during exercise and other conditions that invoke hyperpnoea, the normally thick SA flattens almost to the diameter of the EPPB. Since the resting ostrich has a remarkably slow respiratory rate (six times per minute; e.g.) (Schmidt-Nielsen et al., 1969), it is interesting that an SA should be lacking in this bird. Jones (Jones, 1982a) suggested that the change in the airflow pattern from resting to panting in the ostrich could result from a scaling of the aerodynamic forces that govern flow in extremely large airways. The airflow dynamics in the remarkably large bronchial system of the ostrich may be totally different from those in the lungs of smaller birds.
In conclusion, for a flightless ratite bird, morphologically and morphometrically, the lung of the ostrich appears to present a singular design and exceptional structural refinements. These features conform to the high aerobic capacity attained and sustained by the bird and the thermal extremes that it survives through sustained panting on the ground, without incurring acidbase imbalance of the blood.
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computational fluid dynamics
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