Theta values for C16O18O and C18O2 related to respective pulmonary diffusing capacities

HOME

HELP

FEEDBACK

SUBSCRIPTIONS

SPECIAL COMMUNICATION
Theta values for C¹⁶O¹⁸O and C¹⁸O₂ related to respective pulmonary diffusing capacities

Hartmut Heller and Klaus-Dieter Schuster

Department of Physiology, University of Bonn, 53115 Bonn, Germany

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

The single-breath diffusing capacities for singly and doubly ¹⁸O-labeled CO₂, DL_{C¹⁶O¹⁸O} and DL_C¹⁸O₂,as well as for NO, were determined in seven anesthetized rabbitsto investigate whether the theoretically predicted ratio of specificblood uptake rates of both isotopic CO₂ species, $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}= 2.0, can be derived from the measured values of DL_{C¹⁶O¹⁸O}and DL_C¹⁸O₂. Data of DL were obtained by inflatingthe lungs with gas mixtures containing 0.35% C¹⁶O¹⁸O or 0.8% C¹⁸O₂ or 0.05% NO in nitrogen, with breath-holding periods of 0.05-0.5s and 2-12 s for the CO₂ and NO tests, respectively. $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}was calculated by applying the double-reciprocal Roughton-Forsterequation to DL values obtained in each animal and by assumingthat NO diffusing capacity represents the gas conductance of thealveolar-capillary membrane. The measured ratio was $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}= 1.9 ± 0.2 (mean ± SD), thus comparing reasonably with the predictedone. Therefore, our findings provide evidence that the greatervalue of DL_C¹⁸O₂ is mainly due to the twofoldhigher probability (or theta value) for C¹⁸O₂ than for C¹⁶O¹⁸O to disappear within red blood cells via isotopic exchange reactions.

artificially ventilated rabbits; oxygen-labeled carbon dioxide; single-breath method

	INTRODUCTION

Top Abstract Introduction Methods Results Discussion References

IN PREVIOUS STUDIES (13, 14), singly and doubly ¹⁸O-labeled CO₂, C¹⁶O¹⁸O and C¹⁸O₂, were introduced to determine the pulmonary diffusing capacityfor carbon dioxide in man. The major advantage of this approachis that the rapid dilution of ¹⁸O in the large water pool (55 M) by isotopic exchange betweenCO₂-bicarbonate and water limits the development of significantback pressures of indicator gases within pulmonary capillary blood.The author obtained a ratio of diffusing capacities of the humanlung for C¹⁶O¹⁸O (DL_{C¹⁶O¹⁸O}) and C¹⁸O₂ (DL_C¹⁸O₂) of 1.28.

Because the oxygens in bicarbonate are symmetrical (HC¹⁶O¹⁸O¹⁶O from C¹⁶O¹⁸O and HC¹⁸O¹⁶O¹⁸O from C¹⁸O₂), there is a one in three chance in the case of C¹⁶O¹⁸O but a two in three chance for C¹⁸O₂ that the ¹⁸O label will be in the water pool because of the hydration-dehydrationreactions of CO₂-bicarbonate interconversion that is catalyzedby carbonic anhydrase of red blood cells (RBC) and pulmonary tissue.Because of this twofold higher probability of label removal forC¹⁸O₂ than for C¹⁶O¹⁸O, it was concluded (14) that the estimated difference betweenDL_C¹⁸O₂ and DL_{C¹⁶O¹⁸O}is explainable by a higher kinetics of disappearance via isotopicexchange for C¹⁸O₂ than for C¹⁶O¹⁸O. In addition, the author stated that, by supposing equal diffusionkinetics of both isotopic species and due to DL_C¹⁸O₂>DL_{C¹⁶O¹⁸O}, the value of DL_C¹⁸O₂can be considered to provide a lower limit of the true conductanceof the alveolar-capillary membrane for CO₂.

The present work was undertaken to examine the premises of these interpretations in an animal study. We used the familiardouble-reciprocal Roughton-Forster relationship (12) for dataanalysis

<FR><NU>1</NU><DE>D<SC>l</SC></DE></FR> = <FR><NU>1</NU><DE>Dm</DE></FR> + <FR><NU>1</NU><DE>&thgr; ⋅ Vc</DE></FR> (1)

where DL is the overall pulmonary diffusing capacity for a test gas and the components Dm and $theta$ · Vc represent the true conductanceof the alveolar-capillary membrane and the rate at which the RBCin 1 ml of pulmonary capillary blood will absorb the test gas( $theta$ ) related to the total pulmonary capillary blood volume (Vc),respectively.

If it is true that singly and doubly ¹⁸O-labeled CO₂ diffuse with very similar facility into pulmonary capillary blood (Dm_{C¹⁶O¹⁸O} $approx$ Dm_C¹⁸O₂) but that C¹⁸O₂ is removed within the CO₂-bicarbonate interconversion witha twofold higher probability than C¹⁶O¹⁸O, then $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O} $approx$ 2 should apply. By use of Eq. 1, the ratio of specific uptakerates by RBC for both isotopic CO₂ species can be derived from

(2)

We estimated the membrane diffusing capacity Dm_{C¹⁶O¹⁸O} by calculating Dm_{C¹⁶O¹⁸O}= 12.3 × pulmonary diffusing capacity of NO (DL_NO), falling backon the theoretical prediction that gases permeate lung tissueat rates proportional to their solubilities in the lung [estimatedfrom the solubility constants in water: $alpha$ _CO₂/ $alpha$ _NO = 15.2 (1,17)] and inversely proportional to the square roots of molecularweights ( <RAD><RCD>30</RCD></RAD> / <RAD><RCD>46</RCD></RAD> = 0.81).Because of the very rapid binding of NO to hemoglobin (4, 11),it is usually expected that alveolar-capillary transfer of NOis mainly limited by diffusion (2, 7, 10, 11), leadingto 1/( $theta$ · Vc) $right-arrow$ 0 and DL_NO $approx$ Dm_NO.

We applied the single-breath method to artificially ventilated rabbits to determine values of DL_{C¹⁶O¹⁸O},DL_C¹⁸O₂, and DL_NO. If our assumptions arevalid, the calculated ratio of specific blood uptake rates shouldcompare reasonably with the theoretically predicted value of $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O} $approx$ 2.

	METHODS

Top Abstract Introduction Methods Results Discussion References

Single-breath maneuvers were performed on seven adult Chinchilla cross-breed rabbits weighing 2.8-3.7 kg under pentobarbitalsodium anesthesia (20 mg · kg¹ · h¹ iv). The animals were paralyzed by alcuronium (0.1 mg · kg¹ · h¹ iv), endotracheally intubated (2.5-3.5 mm ID), and artificiallyventilated with room air by a computerized ventilatory servo system.The animals were instrumented with carotid arterial and ear veincannulas for blood gas analyses, determinations of the hemoglobinconcentration of blood ([Hb]), and the administration of drugs.

Test gases. To avoid the formation of oxidation products of NO and to enable the comparison of DL values of the three testgases, three O₂-free gas mixtures, containing 0.35% C¹⁶O¹⁸O or 0.8% C¹⁸O₂ or 0.05% NO in N₂, were prepared and stored in gas-tight flexiblealuminum bags. Pure NO was led through diluted KOH, subsequentlycollected with a KOH-containing syringe, and finally injectedinto the aluminum bags, which had been repeatedly washed out withN₂. To avoid an artificial isotopic exchange with water, pureC¹⁶O¹⁸O or pure C¹⁸O₂ was dried within a trap and led into the N₂-containing aluminumbags.

Protocol of experiments. Before the series of single-breath experiments, pressure-volume curves were recorded. For this purpose,the lungs were inflated and deflated by specific volume stepsand the airway pressure was measured during short breath-holdsby a differential pressure transducer. The residual volume (VR)was set at the lung volume attained at $-$ 20 cmH₂O of airway pressure.It was calculated from the argon (Ar) washout produced by inflatingthe rabbit lungs with the Ar-free test gas mixtures (see Table1). Anatomic and apparatus dead spaces were determined in separateexpirograms for the three test gases and were used to calculatethe effective inflation and deflation times (13).

View this table:
[in this window]
[in a new window]

Table 1. Animal characteristics and experimental parameters

In each animal, the series of C¹⁶O¹⁸O, C¹⁸O₂, and NO experiments were performed in random order, starting the single-breath maneuversfrom VR in each case. The respective times for inflation and deflationwere set at 0.6 s for C¹⁶O¹⁸O and C¹⁸O₂ and at 0.8 s for NO. For the two isotopic CO₂ species, experimentswith breath-holding periods of 0.05, 0.10, 0.15, 0.20, and 0.50s were used to calculate DL (13, 14). The NO single-breathmaneuvers were performed with breath-holding periods of 2, 4,6, 8, and 12 s. The lungs of the rabbits were inflated with 30-47ml of the C¹⁶O¹⁸O- or C¹⁸O₂-containing gas mixtures and with 30-55 ml of the NO-containingtest gas. After breath holding, the total expired gas was sampledby deflating the lungs via a spiral stainless steel tube (3.5mm ID, length 5 m). The gas stored within this tube was driedby freezing and was continuously sucked into the inlet systemof a respiratory magnetic sector mass spectrometer (M3; VarianMAT, Bremen, Germany). As shown in Table 1, the ratio of inflationvolumes for the CO₂ and NO experiments was varied between 0.73and 1.34 to examine the influence of changes in pulmonary capillaryblood volume (and thus of Hb content) on the $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}determinations.

Apart from this gas-sampling procedure, continuous recordings of alveolar partial pressures of O₂ and C¹⁶O₂ (unlabeled CO₂) by mass spectrometry were used to check ventilatoryconditions.

Mass spectrometry. The mass spectrometer used was modified to measure also isotopic ratios (15). The relevant gases NO,O₂, C¹⁶O₂, Ar, C¹⁶O¹⁸O, and C¹⁸O₂ were recorded at two ion collectors and one double collector,which were set at the following mass-to-charge ratios (m/e): 30(NO), 32 (O₂), 44 (C¹⁶O₂), and 46 (C¹⁶O¹⁸O). We determined C¹⁶O₂ at the first plate of the double collector, C¹⁶O¹⁸O at the second plate, and C¹⁸O₂ at the second plate of the same double collector (m/e = 48)by repeatedly changing the accelerating voltage (peak jump). Inthe same way, Ar (m/e = 40) was measured at the C¹⁶O₂ 44-ion collector. To avoid drift errors and cross-talk effects(6, 11, 13), the dry sample gas was repeatedly comparedwith a reference gas that only differed in the content of testgases, and by subtracting the background of the mass peaks. Theconcentrations of C¹⁶O¹⁸O and C¹⁸O₂ were obtained in terms of the difference to natural abundance.The signal-to-noise ratios were 1,656:1 at 3,500 parts per million(ppm) C¹⁶O¹⁸O, 1,905:1 at 8,000 ppm C¹⁸O₂, and 1,351:1 at 500 ppm NO.

Calculations for DL. We used the partial pressures of the three test gases obtained from that end-tidal portion of the gas sample where the concentrationof test gases remained unchanged. These values were processedby applying the DL calculations on the basis of a coupled systemof three differential equations defining gas transfer during inflation,breath holding, and deflation, as previously described in detail(13).

Statistics. Averaged data are given as mean ± SD values. The comparison between the calculated ratios of specific blood uptakerates and the theoretically predicted value $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O} $approx$ 2 was carried out using the Wilcoxon test (one-sample $mu-tilde$ test).Multiple regression analysis was performed on $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}versus [Hb] and ratios of inflation volume.

	RESULTS

Top Abstract Introduction Methods Results Discussion References

Figure 1 shows the time course of alveolar-capillary transfer of test gases in a semilogarithmic plot of ratios of alveolarpartial pressures at overall times t and zero (PA/PA₀) relatedto the overall time period of experiments. PA₀ values were derivedby calculating the dilution of inspired test gases within thealveolar volume (1.5 mmHg < PA_{0,C¹⁶O¹⁸O}< 2.0 mmHg; 4 mmHg < PA_0,C¹⁸O₂ < 5 mmHg; 0.22mmHg < PA_0,NO < 0.26 mmHg). C¹⁶O¹⁸O as well as C¹⁸O₂ were removed according to the following biexponential relationships,where t is time in seconds

P<SC>a</SC>C16O18O/P<SC>a</SC>0,C16O18O = 0.995 ⋅ <IT>e</IT>−3.4 ⋅ <IT>t</IT> + 0.005 ⋅ <IT>e</IT>−0.02 ⋅ <IT>t</IT> (3)

P<SC>a</SC>C18O2/P<SC>a</SC>0,C18O2 = 0.9995 ⋅ <IT>e</IT>−4.6 ⋅ <IT>t</IT> + 0.0005 ⋅ <IT>e</IT>−0.02 ⋅ <IT>t</IT> (4)

but NO disappeared monoexponentially from alveolar space

P<SC>a</SC>NO/P<SC>a</SC>0,NO = 0.93 ⋅ <IT>e</IT>−0.56 ⋅ <IT>t</IT> (5)

During the initial phase (t < 3 s), the ratios of PA to PA₀ of C¹⁶O¹⁸O and C¹⁸O₂ were reduced to less than 0.01 and 0.001, respectively. Thepulmonary diffusing capacities for both CO₂ species were calculatedfrom this fast component by subtracting the partial pressure ofthe remaining residues from the respective PA_{C¹⁶O¹⁸O}values of the fast phase (13, 14). The smallest PA_{C¹⁶O¹⁸O}values, measured during the slow phase (t > 3 s), came close tothe level of natural abundance of C¹⁶O¹⁸O, whereas the smallest PA_0,C¹⁸O₂ values determinedduring the same phase of label removal were 20 times higher thanthe natural C¹⁸O₂ abundance. By contrast to the biexponential kinetics, >99%of the inhaled NO disappeared from alveolar gas after a time periodof 10 s.

View larger version (20K):
[in this window]
[in a new window]

Fig. 1. Semilogarithmic plot of removal of C¹⁶O¹⁸O (+), C¹⁸O₂ ( $open circle$ ), and NO ( $square$ ) from alveolar space versus overall time available for gas transfer (inflation, breath holding, and deflation) obtained from performing 105 single-breath maneuvers on 7 rabbits. Ordinate: log of ratios of alveolar partial pressures at overall times t and zero (PA/PA₀).

The DL data of each rabbit are listed in Table 2. The overall mean ± SD values are DL_{C¹⁶O¹⁸O}= 9.9 ± 1.6 ml · mmHg¹ · min¹, DL_C¹⁸O₂ = 13.3 ± 2.1 ml · mmHg¹ · min¹, and DL_NO = 1.8 ± 0.4 ml · mmHg¹ · min¹. During the single-breath maneuvers and due to the inflationof the rabbit lungs with the O₂-free indicator gas mixtures [VR/inflationvolume = 12.7 ml/(30-55 ml)], the end-tidal PO₂ valuesaveraged 24 ± 4 mmHg. However, after each maneuver the continuousrecording of ventilatory conditions by mass spectrometry showeda fast recovery of alveolar PO₂ to normal values.

View this table:
[in this window]
[in a new window]

Table 2. Single-breath diffusing capacities for C¹⁶O¹⁸O₂, C¹⁸O₂, and NO as well as the corresponding ratio of specific blood uptake rates of both isotopic CO₂ species

By applying Eq. 2 to the individual mean values of DL, we calculated the ratios of specific blood uptake rates of both stableisotopic CO₂ molecules in each rabbit (see Table 2), averaging $theta$ _C¹⁸O₂ / $theta$ _{C¹⁶O¹⁸O} =1.9 ± 0.2. This result is not significantly different from thetheoretically predicted value of $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O} $approx$ 2.0 (Wilcoxon test, $alpha$ = 0.05). Furthermore, there was no dependenceof individual mean values of $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}on the ratios of inflation volume for the CO₂ and NO experimentsand the [Hb] of blood (correlation coefficient of multiple regressionanalysis: 0.503, n = 7, P < 0.6).

	DISCUSSION

Top Abstract Introduction Methods Results Discussion References

The objective of this study was to investigate whether the pulmonary diffusing capacities of the ¹⁸O-labeled stable isotopic species of carbon dioxide, DL_C¹⁸O₂and DL_{C¹⁶O¹⁸O}, reflect the correspondingratio of specific blood uptake rates of both test gases, $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}.Our data provide evidence that the higher kinetics of disappearancefrom alveolar gas found for C¹⁸O₂ compared with C¹⁶O¹⁸O is mainly due to the higher removal rate of C¹⁸O₂ via the above-mentioned CO₂-bicarbonate interconversion. Thisis based on the finding that the calculated ratio $theta$ _C¹⁸O₂/ $theta$ _{C¹⁶O¹⁸O}= 1.9 ± 0.2 compares reasonably with its predicted value (2.0).Because Eq. 2 was applied to data of DL_{C¹⁶O¹⁸O}and DL_NO, the calculation Dm_{C¹⁶O¹⁸O} = 12.3· DL_NO is also confirmed.

The assumption that the pulmonary diffusing capacity of NO should provide a very close estimate of the true conductance ofthe alveolar-capillary membrane has already been used in recentstudies (2, 7, 10, 11). It is mainly based on the observationthat there is a very rapid binding of NO to Hb, the reaction ofwhich is 280 times faster than that of CO (4). Therefore, itwas hypothesized that NO that enters the RBC is almost entirelybound by Hb (11). By taking this aspect into account, as wellas allowing for the fact that NO solubility is greater than O₂solubility, we expect $theta$ _NO values to be >14 ml · ml¹ · mmHg¹ · min¹, as has recently been determined for O₂ (9). This value isgreater than the corresponding value of $theta$ _NO = 4 ml · ml¹ · mmHg¹ · min¹ that can be derived from the study of Carlsen and Comroe (3),who measured red cell kinetics by rapid mixing technique. However,this technique may have been seriously biased by diffusion limitationfrom unstirred layers (9). Therefore, we used $theta$ _NO > 14 ml ·ml¹ · mmHg¹ · min¹ to estimate Dm_NO: on the basis of the double-reciprocal equationof Roughton and Forster (12), the overall mean value of DL_NO= 1.8 ml · mmHg¹ · min¹ found in the present study and a reliable value of pulmonarycapillary blood volume in rabbits, 3 ml, we obtained Dm_NO < 1.9ml · mmHg¹ · min¹. Thus, by using the value of DL_NO, the true NO conductance ofthe alveolar-capillary membrane is, at worst, underestimated by6%.

This evaluation is important to interpreting the deviation between the measured ratio DL_{C¹⁶O¹⁸O}/DL_NO= 5.5 and the theoretically predicted value of 12.3 that wouldapply if the alveolar-capillary transfer of C¹⁶O¹⁸O were also predominantly diffusion limited [1/( $theta$ _{C¹⁶O¹⁸O}· Vc) $right-arrow$ 0]. From the similarity of DL_NO to Dm_NO it can be derivedthat this deviation is mainly caused by a significant contributionof the specific C¹⁶O¹⁸O blood uptake conductance [1/( $theta$ _{C¹⁶O¹⁸O}· Vc)] to the overall resistance to alveolar-capillary transferof C¹⁶O¹⁸O(1/DL_{C¹⁶O¹⁸O}).By using the Roughton-Forster equation again and referring toDm_{C¹⁶O¹⁸O} = 12.3 · DL_NO, one obtains thatthe overall rate of disappearance of C¹⁶O¹⁸O from alveolar space is limited by 55% because of the label removalwithin RBC. The corresponding value for C¹⁸O₂ amounts to 40%.

The RBC act as a sink to remove ¹⁸O-labeled CO₂ via the CO₂-bicarbonate interconversion, and RBC also act as a sink to veryrapidly bind NO to Hb. Therefore, determinations of the single-breathdiffusing capacities of both isotopic CO₂ species and NO mighthave been biased by using different inflation volumes during theCO₂ and NO tests, because pulmonary capillary Hb content changesbecause of various inflation volumes applied to artificially ventilatedanimals (11). Our finding that ratios of theta were independentof variations in inflation volume provides evidence that the specificblood uptake rates of test gases used are much too high to beinfluenced by such variations.

Perspectives

The present animal study revealed that the ratio of pulmonary diffusing capacities of the two ¹⁸O-labeled stable isotopic CO₂ molecules, C¹⁶O¹⁸O and C¹⁸O₂, effectively reflects the difference between the specific blooduptake rates for both isotopic CO₂ species, thus confirming theassumptions previously made (13, 14) with respect to interpretingthe corresponding ratio of diffusing capacities of C¹⁶O¹⁸O and C¹⁸O₂ in man. By using the classical Roughton-Forster equation andan estimated value of the true conductance of the alveolar-capillarymembrane for C¹⁶O¹⁸O, we were able to show that the mean blood uptake resistancesof C¹⁶O¹⁸O and C¹⁸O₂ contribute to the overall resistance to alveolar-capillarygas transfer at levels of 55 and 40%, respectively. In reviewingthe pertinent literature, the latter value (of C¹⁸O₂) compares very closely with the corresponding mean value forCO (42% contribution by blood uptake resistance) that we calculatedfrom studies in humans using 169 subjects (5, 8, 12, 16).Thus we found that the blood uptake resistances to C¹⁸O₂ and CO equally contribute to the corresponding overall resistancesto alveolar-capillary gas transfer.

	ACKNOWLEDGEMENTS

The authors are very grateful for the valuable technical assistance provided by Christa Pusch, Barbara Schreiber, and BerndEixmann.

	FOOTNOTES

Address for reprint requests: H. Heller, Dept. of Physiology, Univ. of Bonn, Nussallee 11, D-53115 Bonn, Germany.

Received 11 August 1997; accepted in final form 21 January 1998.

	REFERENCES

Top Abstract Introduction Methods Results Discussion References

1. Austin, W. H., E. Lacombe, P. W. Rand, and M. Chatterjee. Solubility of carbon dioxide in serum from 15 to 38 C. J. Appl. Physiol. 18: 301-304, 1963[Abstract/Free Full Text].

2. Borland, C. D. R., and T. W. Higenbottam. A simultaneous single breath measurement of pulmonary diffusing capacity with nitric oxide and carbon monoxide. Eur. Respir. J. 2: 56-63, 1989[Abstract].

3. Carlsen, E., and J. H. Comroe. The rate of uptake of carbon monoxide and of nitric oxide by normal human erythrocytes and experimentally produced spherocytes. J. Gen. Physiol. 42: 83-107, 1958[Abstract/Free Full Text].

4. Cassoly, R., and Q. H. Gibson. Conformation, co-operativity and ligand binding in human hemoglobin. J. Mol. Biol. 91: 301-313, 1975[Medline].

5. Cotes, J. E., and A. M. Hall. Normal Values for Respiratory Function in Man. Milan, Italy: Panminerva Medica, 1969, p. 327-343.

6. Gerster, R. Cinétique de l'échange des atomes d'oxygène en phase hétérogène entre C¹⁸O₂ et H₂O. J. Appl. Radiat. Isot. 22: 339-348, 1971.

7. Guénard, H., N. Varène, and P. Vaida. Determination of lung capillary blood volume and membrane diffusing capacity in man by the measurements of NO and CO transfer. Respir. Physiol. 70: 113-120, 1987[Medline].

8. Hamer, N. A. Variations in the components of the diffusing capacity as the lung expands. Clin. Sci. (Colch.) 24: 275-285, 1963.

9. Heidelberger, E., and R. B. Reeves. O₂ transfer kinetics in a whole blood unicellular thin layer. J. Appl. Physiol. 68: 1854-1864, 1990[Abstract/Free Full Text].

10. Manier, G., J. Moinard, P. Téchoueyres, N. Varène, and H. Guénard. Pulmonary diffusion limitation after prolonged strenuous exercise. Respir. Physiol. 83: 143-154, 1991[Medline].

11. Meyer, M., K.-D. Schuster, H. Schulz, M. Mohr, and J. Piiper. Pulmonary diffusing capacities for nitric oxide and carbon monoxide determined by rebreathing in dogs. J. Appl. Physiol. 68: 2344-2357, 1990[Abstract/Free Full Text].

12. Roughton, F. J. W., and R. E. Forster. Relative importance of diffusion and chemical reaction rates in determining rate of exchange of gases in the human lung, with special reference to true diffusing capacity of pulmonary membrane and volume of blood in the lung capillaries. J. Appl. Physiol. 11: 290-302, 1957[Abstract/Free Full Text].

13. Schuster, K.-D. Kinetics of pulmonary CO₂ transfer studied by using labeled carbon dioxide C¹⁶O¹⁸O. Respir. Physiol. 60: 21-37, 1985[Medline].

14. Schuster, K.-D. Diffusion limitation and limitation by chemical reactions during alveolar-capillary transfer of oxygen-labeled CO₂. Respir. Physiol. 67: 13-22, 1987[Medline].

15. Schuster, K.-D., K. P. Pflug, H. Förstel, and J. P. Pichotka. Recent Developments in Mass Spectrometry in Biochemistry and Medicine. New York: Plenum, 1979, p. 451-462.

16. Werner, F., and H. Kolmer. The CO single breath transfer factor of the lung. Pflügers Arch. 393: 269-274, 1982[Medline].

17. Wilhelm, E., R. Baltino, and J. Wilcock. Low-pressure solubility of gases in liquid water. Chem. Rev. 77: 219-262, 1977.

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted
	Citation Map

Services

	Email this article to a friend
	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via Google Scholar

Google Scholar

	Articles by Heller, H.
	Articles by Schuster, K.-D.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Heller, H.
	Articles by Schuster, K.-D.

SPECIAL COMMUNICATION Theta values for C16O18O and C18O2 related to respective pulmonary diffusing capacities

SPECIAL COMMUNICATION
Theta values for C¹⁶O¹⁸O and C¹⁸O₂ related to respective pulmonary diffusing capacities