ABSTRACT
The unidirectional flow through the gas-exchanging bronchi of bird lungs is known to be effected by (1) the structure of the major bronchi and (2) a pressure difference between the cranial and caudal air sacs.
To study the effects of bronchial structure, simple physical models of bird lungs were constructed. They suggested that, to achieve unidirectional flow, air in the caudal portion of the primary bronchus must be directed towards the orifices of the mediodorsal bronchi.
To study the effect of air sac pressures, a controllable pressure difference was produced between the air sac orifices of fixed duck lungs. The cranial orifices had a higher pressure than the caudal ones during inhalation and vice versa during exhalation. There was a set of pressure differences for which the paleopulmo received the same flow rate during inhalation as during exhalation. High pressure differences caused more flow in the paleopulmo during exhalation than during inhalation; low pressure differences had the converse effect.
Introduction
Although birds inspire and expire, flow through most of their gas-exchanging bronchi is unidirectional. Obtaining unidirectional flow from bidirectional flow requires a mechanism equivalent to a set of valves. The nature and location of the valving mechanism of bird lungs, despite much investigation, remains enigmatic.
Dotterweich (1936) proposed hydrodynamic valving, since he could not find the flap valves proposed by earlier authors (Brandes, 1924; Bethe, 1925; Vos, 1934). Hazelhoff (1943) advanced the hydrodynamic theory by producing unidirectional flow in dead birds and in a glass model of bird lungs. The details of the flow pattern in the major bronchi and air sacs (Fig. 1) were not elucidated until the work of Schmidt-Nielsen et al. (1969), Bretz & Schmidt-Nielsen (1971, 1972), Scheid & Piiper (1971), Brackenbury (1971) and Bouverot & Dejours (1971). A detailed history of the considerable body of additional literature is provided by Scheid (1979).
In the present paper, the flow pattern for the respiratory system shown in Fig. 1 is called the ‘standard’ flow pattern. Although this pattern is agreed to be the basic one, there may, on occasion, be flow in those bronchi marked with stars in Fig. 1 (Powell, Geiser, Gratz & Scheid, 1981; Bretz & Schmidt-Nielsen, 1971). There are also some parabronchi in any bird to which this flow pattern is not applicable (Duncker, 1971; Scheid, Slama & Piiper, 1972).
The valving mechanism appears to involve (1) some structural feature(s) of the major bronchi and (2) a difference in pressure between the cranial and caudal air sacs. The importance of structural features was demonstrated by Hazelhoffs (1943) glass model. This faithfully reproduced some structural features of bird bronchi, such as the guiding dam (Fig. 1) that he proposed as the cause of unidirectional flow, but omitted the cranial air sacs. The preserved lungs used by Scheid et al. (1972) also demonstrated the importance of structural features. They produced unidirectional flow with their air sac orifices all at the same pressure. In contrast to the work of these authors, Brackenbury (1971, 1972a,b, 1979) maintained that the flow pattern is caused by pressure differences. Brackenbury (1971) found the pressure in the caudal air sacs to be lower during inhalation and higher during exhalation than in the cranial air sacs.
To study the effect of bronchial structure, a simple physical model that would reproduce the essential features of the standard flow pattern was developed. Aspects of the geometry in subsequent models were altered to see if changes in the flow pattern could suggest how structural features interacted with the passage of air to cause the unidirectional flow.
To study the effect of air sac pressure differences, a controllable pressure difference between the air sac orifices of fixed duck lungs was produced. Pressures in the caudal air sac orifices were lower during inhalation and higher during exhalation than in the cranial air sac orifices. To assess the resulting flow pattern, the flow rate through the paleopulmo was ascertained by measuring the pressure drop between a mediodorsal bronchus and a medioventral bronchus. The pressure drop between the two bronchi was calibrated against the flow rate through the whole paleopulmo.
Materials and methods
Obtaining lungs
The lungs of four freshly killed adult Pekin ducks (Anas platyrhynchos, 2·7-2·9 kg in mass) were fixed in situ by blowing formaldehyde vapour through the trachea after the viscera had been removed and the air sacs slit. After fixation, the lungs, dorsal ribcage and associated vertebrae were isolated intact. The lung from only one side of a bird was used. All openings to the lung on the opposite side were blocked with silicone rubber (Dow Corning, cat. no. 8641). The diameters of the primary bronchi (measured 1 cm external to the lung) ranged from 5 to 7 mm.
Pressure and flow rate measurement
Pressure differences were measured with a Datametrics 570D-10T-2A1-VIX Barocel pressure transducer and a Datametrics 1174-B1A-5A1-A1-4·75 electronic manometer. The stated bias of less than 0·0025R+0·267 (where R is the reading in Pa) was verified for pressure differences from 9·81 to 29·3 (±0·27) Pa by comparison with measurements using a multiplying manometer (see Vogel, 1981). Data were not adjusted for the pressure difference, less than 0·2 Pa, resulting from the height difference between the openings of the cannulae. A constant air flow (between 1 and 30cm3s-1) was either pumped into the primary bronchus (inspiration) or withdrawn from it (expiration). The worst case error in measuring flow rates was less than 0·85 cm3 s-1 (calculation appears in Kuethe, 1986).
Calibrating the paleopulmo for use as a flow meter
Sixteen gauge hypodermic needles were inserted at each end of a small set of parabronchi. One was inserted three-quarters of the distance from the primary bronchus along the second mediodorsal bronchus (D in Fig. 2A). The second was inserted in the first medioventral bronchus at the position where cigar smoke appeared when blown through the first cannula (V in Fig. 2A).
The primary bronchus was blocked with a balloon between the orifices of the medioventral and mediodorsal bronchi (see Graf, Molony & Scheid, 1976), and the cranial air sac orifices were blocked with silicone rubber so that all the measured flow through the primary bronchus went through the paleopulmo (see Fig. 2A). The flow rate through the paleopulmo was plotted against the pressure drop from D to V to give the calibration graph (Fig. 3). For the purpose of this graph, so-called dynamic pressure effects which must be avoided when measuring resistances (as in Macklem, Bouverot & Scheid, 1979) were of no concern, as long as every time a given flow rate occurred in the paleopulmo the same pressure reading was obtained. The same pressure readings were obtained whether the caudal thoracic or abdominal sac orifice was blocked, or both were open.
Data collection from fixed lungs
The cranial sac orifices opened into a hollow dome of silicone rubber, whereas the caudal air sac orifices were left open to the atmosphere (Fig. 2B). The interior of the dome communicated with the atmosphere through a short hose whose resistance could be varied with a screw clamp. This resistance ensured that, when the lung was ventilated through the primary bronchus, the cranial air sac pressure was higher during inhalation and lower during exhalation than the caudal air sac pressure. Pressure differences were similar to those measured in live birds (Brackenbury, 1971; Kuethe, 1986).
Experimental data consisted of (1) the pressure drop from D to V (see Fig. 2B) obtained at different flow rates through the primary bronchus, which monitors flow through the paleopulmo, and (2) and pressure difference between AAS and PAS in Fig. 2B at different flow rates, which represents the difference in pressure between the cranial and caudal air sacs. During data collection, the primary bronchus was unobstructed (Fig. 2B).
The effects of three different air sac pressure differences on the flow in the paleopulmo were ascertained using three hose resistances. At each hose resistance flow data were collected for at least nine inspiratory and nine expiratory flow rates; air sac pressure data were collected for at least seven inspiratory and seven expiratory flow rates. The first resistance was such that the flow in the paleopulmo (indicated by the pressure drop from D to V in Fig. 2B) was the same during inhalation as during exhalation. The second resistance was higher than the first, giving more extreme air sac pressure differences. The third resistance was lower than the first, giving less extreme air sac pressure differences.
Since it was necessary to verify the position of the balloon (which was used only during calibration) by dissection, in practice the calibration was performed after the data collection.
Models
Clear plastic models were constructed using polymethylmethacrylate. Cut pieces were sandwiched between two solid sheets so that passages had rectangular cross-sections. The primary bronchus of the models was 9 mm x 10 mm. The models had one orifice for the cranial air sacs, one for the caudal air sacs and one for the primary bronchus. The parabronchi of the paleopulmo were represented by one passage connecting a single mediodorsal bronchus to a single medioventral bronchus.
A short hose was attached to the cranial sac orifice to create a pressure difference just as for the fixed lungs. The models were submerged in a basin of water and water was passed through their primary bronchi (steady flows of 0·1-15 cm3 s-1). The flow pattern was observed with Evans blue dye. Flow rates were estimated to within a factor of two.
For flow in the models to represent flow in the lungs, the Reynolds number (Luρ/μ) must be the same for both situations (see Batchelor, 1967). For both fixed lungs and models, the length (L) was taken as the square root of the cross-sectional area of the primary bronchus; the speed, u, was the flow rate through the primary bronchus divided by the cross-sectional area of the primary bronchus; ρ was the density; and μ was the viscosity of the fluid.
The Reynolds numbers (Re) for the models ranged from 9 to 1400, and for the fixed lungs from 12 to 370. The Reynolds number for a 2·8-kg duck ranged from 66 to 660 (resting to 10 times resting ventilation rate as calculated from the data of Lasiewski & Calder, 1971).
Results
Fixed lungs
In Fig. 4, A, B and C give the flow rates through the paleopulmo (the pressure drop from D to V in Fig. 2B was converted to flow rates using the calibration curve, Fig. 3) and D, E and F give the pressure differences between the air sacs (between AAS and PAS in Fig. 2B). The pairs A, D; B, E and C, F represent the three experimental conditions of air sac pressure differences (see Materials and methods). In A, B and C, the dashed line labelled 100 % represents the same flow rate of air passing through the paleopulmo in the correct direction as is passing through the primary bronchus. The dashed line labelled 50 % represents half of the total flow rate going through the paleopulmo as is passing through the primary bronchus. The air flow was unidirectional in the paleopulmo for all the flow rates and air sac pressure differences, except for flow rates below 8 cm3 s−1 in Fig. 4C.
To be consistent with the standard flow pattern, the flow rate through the paleopulmo during inhalation plus the flow rate through the paleopulmo during exhalation should equal the flow rate on the 100 % line (their average should fall on the 50 % line). In Fig. 4A-C, when the flow rate in the primary bronchus was below 15cm3s-1, not enough air was passing through the paleopulmo to be consistent with the standard flow pattern. As the flow rate increased towards 30cm3s-1, the average of the paleopulmo flow rates during inhalation and exhalation came closer to the 50 % line.
The difference in the air sac pressures affected the relative amount of flow in the paleopulmo during inhalation and exhalation. For the pressure differences in Fig. 4D, the flow rates were approximately equal. For pressures only 5 % higher (Fig. 4E rather than Fig. 4D), there was noticeably more air going through the paleopulmo during exhalation than during inhalation (Fig. 4B). When the pressure differences were lower (Fig. 4F rather than Fig. 4D), the flow through the paleopulmo was higher during inhalation than during exhalation (Fig. 4C).
Models
Flow patterns obtained in four different models at a flow rate of 10cm3s-1 of water (Re = 930) are shown in Fig. 5. The model in Fig. 5A had the standard flow pattern. Modifications of this model either maintained the standard flow pattern (as in Fig. 5C) or failed to produce the standard flow pattern (as in Fig. 5B,D).
Changing the resistance of the hose to the cranial air sac orifice, and thus changing the pressure difference between the air sac orifices, had a similar effect as in the fixed lungs. When the hose was constricted relative to the position resulting in the flow pattern shown in Fig. 5A,C, more water passed through the paleopulmo during exhalation than during inhalation. When it was loosened, more water passed through the paleopulmo during inhalation than during exhalation.
As in the fixed lungs, the model shown in Fig. 5A became less effective at valving at slower flow rates. However, with the model, it was possible to see the alterations in flow pattern. At 7cm3s-1, water ‘leaked’ through the proximal medioventral bronchus during inhalation and through the primary bronchus during exhalation. This leakage became more severe as the flow rate was slowed, until at l·5cm3s-1, there was no flow through the paleopulmo during inhalation. At 0·5 cm3 s−1, water was observed passing through the paleopulmo in the wrong direction during inhalation.
Discussion
In a fixed lung, even if the flow rates through the paleopulmo are consistent with the standard flow pattern, it cannot be known for certain that the lung has the standard flow pattern. To draw this conclusion, one would need to know that the flow rate through the cranial air sac orifices was the same as the paleopulmo flow rate during inhalation, and the same as the primary bronchus flow rate minus the paleopulmo flow rate during exhalation. Even though the complete flow pattern is not known, the data (Fig. 4) support Brackenbury’s (1971, 1972a,b, 1979) claim that the flow pattern is dependent on the pressure difference between the cranial and caudal air sacs. The relative flow in the paleopulmo during inhalation compared with exhalation appears to be controlled by this pressure difference.
It should be noted that the steady flows used in this study are simpler than the tidal flows found in live birds. Thus, the Reynolds numbers and pressure differences at which given flow patterns occur may not be comparable with those of live birds. Although the pressure differences between the experimental ‘air sacs’ were of the same order of magnitude as those in live birds [present study: 0-60 Pa for fixed lungs with steady flow; Brackenbury (1971), 0-5 Pa between caudal thoracic and clavicular sacs of an anaesthetized goose, 2·4—4·7 kg in mass; Kuethe (1986), 0-200 Pa between caudal thoracic and clavicular sacs, and 0-100 Pa between the abdominal and clavicular or between the cranial thoracic and caudal thoracic sacs of conscious ducks, 2·7-2·9kg in mass], one cannot be sure that the pressure differences reported for the fixed lung would occur in a live duck, even if at a given instant the duck had the same flow rates and flow pattern as the fixed lung.
The valving demonstrated by the crude models bears a remarkable functional similarity to the unidirectional flow in birds lungs, although the models did not valve as effectively as the fixed lungs. Despite the similarities of the flow patterns, there are obvious differences in geometry and compliance between the models and bird lungs, and obvious differences between the steady flow employed in this study and the tidal flow in birds. Given these differences, it must remain unclear whether the models, or even the fixed lungs, operate with the same mechanisms as live birds.
However, the models suggest that the fluid in the caudal portion of the primary bronchus needs to be guided by some structural feature towards the orifices of the mediodorsal bronchi, as suggested by Hazelhoff (1943). However, Hazelhoffs dam per se may not be responsible for the valving. When it was excised from one of the fixed duck lungs, the lung was still capable of valving. The only difference in its behaviour was that for the same relative flow rates in the paleopulmo, a different set of air sac pressure differences was required (data appear in Kuethe, 1986). Apparently, when Hazelhoffs dam is removed from a duck lung, the air is still guided towards the mediodorsal bronchi.
The models and fixed lungs suggest how fluid momentum and air sac pressures might interact to produce the flow pattern in the absence of Hazelhoffs dam. During inhalation, air must flow around a bend to enter the caudal air sacs, whether Hazelhoffs dam is present or not. In general, the pressure on the outside of a bend is higher than the pressure on the inside. The pressure difference represents the force which changes the fluid’s momentum. The openings of the mediodorsal bronchi are on the outside of the bend. The pressure difference around this bend, together with other manifestations of the air’s inertia, might explain the valving. During inhalation the pressure difference created by the bend opposes the pressure difference between the air sacs. The bend pressure difference is high enough to create a net force driving fluid from the mediodorsal bronchial orifices towards the medioventral bronchi. The inertia of the air in the primary bronchus tends to prevent it from changing momentum and entering the medioventral bronchi directly. During exhalation the pressure difference between the air sacs favours the flow from mediodorsal bronchi to medioventral bronchi. The inertia of the air from the caudal sacs tends to prevent it from changing momentum and flowing directly into the primary bronchus.
Because this scheme depends on inertia, the valving should be less effective at lower flow rates (recognized by Dotterweich, 1936; Hazelhoff, 1943), as indeed it was in both fixed lungs and models.
ACKNOWLEDGEMENTS
I thank Knut Schmidt-Nielsen for philosophical advice, Steven Vogel for helping me transform my dissertation into a paper and Knut Schmidt-Nielsen, Sharon Gowan and Ira Warrenfelt for help with earlier versions. This work was supported by NIH grant no. HL02228.