key: cord-0021779-4swdjbed
authors: Svedmyr, Anders; Konrad, Mark; Wallin, Mats; Hallbäck, Magnus; Lönnqvist, Per-Arne; Karlsson, Jacob
title: Non-invasive capnodynamic mixed venous oxygen saturation during major changes in oxygen delivery
date: 2021-10-05
journal: J Clin Monit Comput
DOI: 10.1007/s10877-021-00762-5
sha: e304dfa91e19918bd88a61a8a0125eb83bde4edc
doc_id: 21779
cord_uid: 4swdjbed

Mixed venous oxygen saturation (SvO(2)) is an important variable in anesthesia and intensive care but currently requires pulmonary artery catheterization. Recently, non-invasive determination of SvO(2) (Capno-SvO(2)) using capnodynamics has shown good agreement against CO-oximetry in an animal model of modest hemodynamic changes. The purpose of the current study was to validate Capno-SvO(2) against CO-oximetry during major alterations in oxygen delivery. Furthermore, evaluating fiberoptic SvO(2) for its response to the same challenges. Eleven mechanically ventilated pigs were exposed to oxygen delivery changes: increased inhaled oxygen concentration, hemorrhage, crystalloid and blood transfusion, preload reduction and dobutamine infusion. Capno-SvO(2) and fiberoptic SvO(2) recordings were made in parallel with CO-oximetry. Respiratory quotient, needed for capnodynamic SvO(2), was measured by analysis of mixed expired gases. Agreement of absolute values between CO-oximetry and Capno-SvO(2) and fiberoptic SvO(2) respectively, was assessed using Bland–Altman plots. Ability of Capno- SvO(2) and fiberoptic SvO(2) to detect change compared to CO-oximetry was assessed using concordance analysis. The interventions caused significant hemodynamic variations. Bias between Capno-SvO(2) and CO-oximetry was + 3% points (95% limits of agreements – 7 to + 13). Bias between fiberoptic SvO(2) and CO-oximetry was + 1% point, (95% limits of agreements − 7 to + 9). Concordance rate for Capno-SvO(2) and fiberoptic SvO(2) vs. CO-oximetry was 98% and 93%, respectively. Capno-SvO(2) generates absolute values close to CO-oximetry. The performance of Capno-SvO(2) vs. CO-oximetry was comparable to the performance of fiberoptic SvO(2) vs. CO-oximetry. Capno-SvO(2) appears to be a promising tool for non-invasive SvO(2) monitoring. SUPPLEMENTARY INFORMATION: The online version contains supplementary material available at 10.1007/s10877-021-00762-5.

Mixed venous oxygen saturation (SvO 2 ) is a clinically useful monitoring parameter that provide important information regarding the whole-body oxygen delivery/consumption balance and is of particular interest in the setting of anaesthesia and intensive care [1] . The use of SvO 2 as a routine monitoring parameter has so far been hampered by the fact that intermittent blood sampling from the pulmonary artery (CO-oximetry; representing "gold standard") as well as continuous assessment by fibreoptic spectrophotometry both require invasive catherization of the pulmonary artery, which is associated with certain risks as well as increased nursing care demands and cost [2, 3] .

During our development of a modern version of capnodynamic assessment of cardiac output (Effective Pulmonary Blood Flow, CO EPBF ), which we have found to produce similar results when compared to accepted reference methods, we have come to realize that combining CO EPBF with the respiratory quotient (RQ) results in the possibility to determine SvO 2 noninvasively [4] [5] [6] [7] . In a recent proof-ofconcept study we have found that this new non-invasive and continuous methodology of monitoring SvO 2 (Capno-SvO 2 ) show promising results when compared to CO-oximetry determinations of SvO 2 in a porcine model, during modest hemodynamic challenges [8] .

The aim of the present study was to validate Capno-SvO 2 against the gold standard CO-oximetry for agreement of absolute values and ability to detect change during profound variations in oxygen delivery while measuring RQ, using our previously well-established porcine model. A comparison between CO-oximetry and another continuous SvO 2 methodology, i.e., fibreoptic SvO 2, was also included for comparison.

The study was performed at the Hedenstierna Laboratory, Uppsala University, Uppsala Sweden. Authorization was granted from Uppsala Animal Ethics Committee (Uppsala, Sweden case number C75/16, chairperson Erik Göransson on August 26, 2016) .

The animals were handled in accordance with the animal experimentation guidelines of the Uppsala Animal Ethics Committee and Animal Research: Reporting of In Vivo Experiments (ARRIVE) guidelines.

Eleven domestic-breed pigs of both sexes (median weight 29.6 kg, range 27.1-31.7 kg, 6-8 weeks of age), from the same breeding colony (Mångsbo Farm, Uppsala, Sweden) were used. The animals were kept in a light-and temperature-controlled environment, with unlimited access to tap water and food on a standardized schedule. The experiments were done during daytime hours.

The pigs were anaesthetized as previously described and mechanically ventilated in a volume-controlled mode (Servo-I; Maquet, Solna, Sweden), with tidal volume of 10 mL kg −1 and fraction of inspired oxygen (FiO 2 ) 0.3 [9] . Positive end-expiratory pressure (PEEP) was kept at 5 cm H 2 O after an initial 2-min period of lung expansion using PEEP 10 cm H 2 O as previously described [8] . After the lung expansion manoeuvre, an air test using FiO 2 0.21 was performed and repeated if necessary, aiming for sustained pulse oximetry saturation > 97% as indicative of open lung conditions [10] . The animals were given a bolus of Ringers' acetate solution 20 mL kg − 1 after induction and thereafter kept on maintenance infusion of glucose 25 mg mL −1 8 mL kg −1 h −1 and Ringer's acetate solution 10 mL kg −1 h −1 . Exhaled CO 2 was measured by a mainstream infrared CO 2 sensor (Capnostat-3; Respironics Inc, Wallingford, CT), and ventilation airflow was registered through the regular flow sensor of the servo-I ventilator. Volumetric capnography was utilised for calculating the CO 2 elimination rate (VCO 2 ), as described in previous studies [11] . Adequate anesthetic depth and analgesic level were tested regularly during the experiment according to standard procedures of the laboratory. The animals were fitted with monitoring devices described in detail in previous studies [9] . In addition a 7.5 F pulmonary artery catheter with fibreoptic SvO 2 monitoring (Swan-Gantz pulmonary artery catheter, model 774F75; Edwards Lifesciences, Irvine CA; USA) and a 5 F femoral artery cannula for transpulmonary thermodilution cardiac output monitoring (PICCO2™, Pulsion Medical Systems, Munich, Germany), were also included as well as an additional 7.5 F pulmonary artery introducer sheath for rapid fluid administration.

A 12 F balloon tipped catheter (Mediq Sverige AB, Uppsala, Sweden) was surgically introduced through the left femoral vein, to a depth of 30 cm corresponding to the inferior vena cava (IVC). The catheter was fitted with a 10 mL balloon allowing partial IVC occlusion when inflated with NaCl 0.9%. The animals were given a bolus dose of intravenous heparin 5000 U (LEO pharma) to minimize the risk of clotting due to the extensive intravascular monitoring setup. SvO 2 through blood samples were analysed by a COoximeter calibrated for porcine hemoglobin (OSM3; Radiometer Medical AbS, Brønshøj, Denmark). This also provided the hemoglobin level, necessary for the calculations of CO EPBF and Capno-SvO 2 as well as for calibrations of fiberoptic SvO 2 .

The principle behind continuous Capno-SvO 2 method has been described in detail in previous work by our research team [8] . The Capno-SvO 2 method is based on the differential Fick principle and utilizes a combination of continuous estimation of CO EPBF and oxygen consumption (VO 2 ) incorporated in a rearranged Fick's equation [12] . CO EPBF is estimated by applying a special breathing pattern of variations in I:E relationships (six breaths with normal I:E relations followed by three breaths vid an approximately 2 s expiratory pause). This breathing pattern causes small fluctuations in alveolar CO 2 concentration and VCO 2 , related to the pulmonary blood flow participating in gas exchange which allows for estimation of CO EPBF [5, 7, 13] . VO 2 can be estimated using continuous volumetric capnography measurement of VCO 2 combined with RQ:

where VO 2 is the oxygen consumption (mL min − 1 ), VCO 2 is the CO 2 production rate (mL min − 1 ), RQ is the respiratory quotient.

(1) VO 2 = VCO 2 RQ VCO 2 applied in Eq. 1 is determined as a moving mean value of measured CO 2 elimination made over a period of 20 min in order to produce stable VCO 2 values with the intent to reflect an assumed stable metabolism.

Using Fick's equation for oxygen, the content of oxygen in mixed venous blood (CvO 2 ) can be derived:

where CO EPBF is the effective pulmonary blood flow (L min − 1 ), VO 2 is the oxygen consumption (mL min − 1 ), CcO 2 is the pulmonary end capillary oxygen content (mL L − 1 ), CvO 2 is the pulmonary mixed venous oxygen content (mL L − 1 ). Equation 2 can be further rearranged to derive CvO 2 :

where CO EPBF is the effective pulmonary blood flow (L min − 1 ), VO 2 is the oxygen consumption (mL min − 1 ), CcO 2 is the pulmonary end capillary oxygen content (mL L − 1 ), CvO 2 is the pulmonary mixed venous oxygen content (mL L − 1 ). CvO 2 from Eq. 3 can then be used to calculated SvO 2 by using the solubility constant for oxygen in blood plasma, Hüfner's constant and the hemoglobin value as previously described thereby generating breath-by-breath estimations of SvO 2 [8] .

The RQ was determined immediately before the start of the first challenge (morning) and immediately before the start of the last challenge (afternoon), approximately 4 h apart (shown in Fig. 1 ). Measurements were performed in all animals, by analysis of mixed expired gas collected in a Douglas bag. Each RQ measurement was conducted in the following way:

• Ventilator bias flow during expiration phase ((normally 2 L min −1 in Servo-I ventilator (Maquet, Solna, Sweden))

was turned off to avoid diluting the gas in the bag with inspiration gas. • FiO 2 was changed from 0.30 to 0.21 (i.e., room air), which was done for two reasons; it gives the best conditions for the RQ calculation (as shown in Eq. 1 below) and the inspired gas concentration is well-defined without relying on accurate gas mixing by the ventilator. • To reach a stable state of nitrogen (N 2 ), 20 min wash-in of N 2 was allowed after the change of FiO 2 and before the bag was connected to the ventilator exhaust port. • Gas was collected for about 10 min; roughly 70 L of expiratory gas was collected. • The content of the bag was analyzed using the sidestream gas analyzer of a Flow-i anesthesia system (Maquet, Solna, Sweden). Gas was alternatingly sampled from the bag or from the room air.

Gas concentrations of FiO 2 (room air), FemixO 2 (bag) and FemixCO 2 (bag) were measured at ATPD state (Ambient temperature and pressure, dry). RQ was calculated using the following formula, which is based on the Haldane transformation to account for the imbalance between inspiration and expiration volumes:

RQ is the respiratory quotient, FiO 2 is the fraction of inspired oxygen, FemixCO 2 is the carbon dioxide concentration in the Douglas bag, FemixO 2 is the oxygen concentration in the Douglas bag.

A detailed derivation of the RQ-equation can be found in Supplemental Description Content 1.

After preparation, the animals were allowed a 20-minute stabilizing period. Following this, an arterial blood sample was taken for calibration of the fiberoptic (Hb and CO-oximetry SvO 2 as per the manufacturers recommendation) and the capnodynamic monitoring system (Hb). Subsequently, five paired baseline measurement of all three methods were performed, 1 min apart, for calculation of

Scheme of the study protocol. RQ respiratory quotient; (FiO 2 ), FiO 2 steps. Black arrows indicate calibration points were fiberoptic SvO 2 was calibrated against CO-oximetry and hemoglobin and Capno-SvO 2 against current hemoglobin inherent precisions. After this, the animals were subjected to six different hemodynamic challenges anticipated to affect SvO 2 ( Fig. 1 fused back over 5-10 min and SvO 2 data were recorded before transfusion and 0, 5, 10, 15 and 20 min after completion of the transfusion where 0 is just after completed infusion. 5. Cava balloon: the cava balloon was inflated (reducing cardiac output by 30-50%). SvO 2 data was collected prior to inflating the balloon, 2 min after inflation, and 3 min after deflation. 6. Dobutamine: a central infusion of dobutamine (Hameln pharma gmbh, Hameln, Germany) 10 mcg kg −1 min −1 was started immediately after the 3-min recording after cava balloon deflation. SvO 2 was then recorded 5, 10 and 15 min after starting the dobutamine infusion.

The fiberoptic SvO 2 measurement was calibrated with Hb-level and CO-oximetry SvO 2 values as per manufacturer's instructions. This was performed totally 4 times during the experiment as marked in Fig. 1 to ensure continuous optimal performance during the experiment. At the same time points, the capnodynamic method was calibrated with the corresponding Hb-level. Throughout the study protocol, Capno-SvO 2 and fiberoptic SvO 2 , were recorded just before the blood samples for CO-oximetry were drawn. Due to previous experiences from caval occlusion causing extensive hemodynamic strain on the animals, no baseline recordings were made before the dobutamine step. Instead, dobutamine was started immediately after the last recording of step 5 as described above. The 3-minute recordings after cava balloon deflation, i.e., just before start of the dobutamine infusion, was used as comparison point for concordance analysis for the dobutamine step.

The animals were euthanized at the end of the experiment, according to the laboratory's routines.

Raw data for absolute values of all three SvO 2 methods (CO-oximetry, Capno-SvO 2 and fibreoptic SvO 2 ), as well as paired differences between Capno-SvO 2 and CO-oximetry and between fibreoptic SvO 2 and CO-oximetry, were controlled for normal distribution by D'Agostino and Pearson test and visual inspection of the corresponding histograms. Values are presented as mean and 95% confidence interval (CI).

The first five measurements, during hemodynamically stable baseline conditions, were used for calculation of inherent precision for each SvO 2 method respectively. Inherent precision was defined as 2 times the coefficient of variation (CV = SD/mean) and was in turn used to quantify the least significant change (LSC) for the reference method CO-oximetry [14] . The LSC reflects the minimum change measured and recognized as a true change [14] . LSC was then used to determine the exclusion zone in the concordance analysis as previously described [8] .

Bland-Altman analysis corrected for repeated measurements was used to assess agreement of absolute values between paired recording of CO-oximetry and Capno-SvO 2 as well as between CO-oximetry and fibreoptic SvO 2 . Bias was defined as the mean difference between the tested methods and the reference method [15, 16] . Limits of agreement (bias ± [1.96 × SD]) were used when presenting the spread of included data points and are shown with the corresponding 95% CI. Mean percentage error (PE) was calculated as 1.96 × SD of the differences, divided by the mean of the reference method [17] . A predefined PE of < 30% was defined a priori to indicate a clinically useful agreement. The predefined maximum allowed difference for agreement between the tested methods and the reference method was set to 15% points (based on previous published performance of fibreoptic SvO 2 devices and Capno-SvO 2 ) [8, [18] [19] [20] . Based on our previous study, given the maximally allowed difference between the tested method and the reference method, a minimum of approximately 250 paired data points (corresponding to 10 animals with 25 paired recording per animal) was required to show that the 95% confidence interval of the limits of agreement would fall within the pre-defined maximal allowed difference thus showing that the methods are in agreement (80% power, 0.05 significance level) [8, 15, 21] . The ability of Capno-SvO 2 and fibreoptic SvO 2 to track changes in SvO 2 compared to the refence method, was assessed by calculating the concordance rate, i.e., the percentage of data points moving in the same direction when comparing two different techniques [22] . Recorded changes between baseline measurements before each hemodynamic intervention, and the value corresponding to the highest change from baseline within that intervention, were used for calculation of the concordance rate. The LSC for COoximetry was found to be 9.5%. Based on this, changes in SVO 2 of less than 9.5% (rounded up to 10%) of the mean of all SvO 2 CO-oximetry recordings (corresponding to a minimal change in CO-oximetry SvO 2 of 5% points) were not regarded as true changes and excluded from the concordance analysis [14] .

Due to the increasingly unreliable performance of CO-oximetry method for low SvO 2 levels, i.e., for values under 30%, CO-oximetry SvO 2 values under 30% and its associated Capno-SvO 2 and fibreoptic SvO 2 values were excluded in the analysis [23, 24] .

GraphPad Prism (version 9.0.0 for Windows, GraphPad Software, San Diego, CA, USA) and Medcalc Statistical Software version 16.8.4 (MedCalc Software, Ostend, Belgium) was used for statistical calculations and Microsoft Excel for Mac 2020 version 16.41 for data handling.

All animals survived the experiment. SvO 2 data for step 1-3 in the protocol was excluded from one animal due malposition of the PA-catheter which was then repositioned correctly for step 4-6. The dobutamine step was introduced after the first animal and thus includes only 10 animals.

The inherent precision was found to be ± 7% for CO-oximetry SvO 2 and ± 8% and ± 6% for Capno-SvO 2 and fiberoptic SvO 2 , respectively which is in line with previous publications [8, 19] .

The mean RQ for morning and afternoon recordings for all eleven animals, i.e., in total 22 RQ values, was found to be 0.97 (range 0.88-1.06) and RQ 0.97 was then used for all SvO 2 -capno calculations.

All animals displayed SvO 2 reactions in an anticipated manner when exposed to the various hemodynamic interventions. Both Capno-SvO 2 and fiberoptic SvO 2 showed parallel changes when compared to the reference method CO-oximetry with increase in SvO 2 in response to increased FiO 2 , crystalloid infusion, blood transfusion and dobutamine administration. Correspondingly, hemorrhage and partial cava occlusion led to decreases in SvO 2 for all methods. The changes in SvO 2 for each hemodynamic intervention for all three SvO 2 methods are shown in the event plot in Fig. 2 

Bland-Altman analysis for all paired data showed a bias between Capno-SvO 2 and CO-oximetry of + 3% points with 95% limits agreement of -7 (CI − 10 to -4) to + 13 (CI 11 to 17) percentage points and a mean percentage error of 18%. Correspondingly, the bias between fiberoptic SvO 2 and CO-oximetry was found to be + 1% point with 95% limits of agreement of − 7 (CI − 8 to − 6) to + 9 (CI 8 to 11) percentage points and PE 16%. Bland Altman plots for Capno-SvO 2 vs. CO-oximetry and fiberoptic SvO 2 vs. CO-oximetry are shown in Fig. 3 . Table 1 shows the agreement of absolute values between the reference method and the tested methods for each hemodynamic intervention.

The trending ability for Capno-SvO 2 and fiberoptic SvO 2 , compared to CO-oximetry, are presented as four-quadrant plot illustrations in Fig. 4 .

For Capno-SvO 2 , a total of 45 data points were found to lie outside the predefined 10% exclusion zone. 44 out of 45 values changed in the same direction as the reference method CO-oximetry which generates a concordance rate of 98%. The corresponding data for fiberoptic SvO 2 was 46 data points outside the exclusion zone with 43 data points moving in the same direction as the reference method i.e., a concordance rate of 93%. Table 1 Bias and limits of agreement between Capno-SvO 2 and CO-oximetry SvO 2 as well as between fiberoptic and CO-oximetry SvO 2 for the various hemodynamic challenges 

The main finding of the current study was that Capno-SvO 2 generates absolute values close to the gold standard COoximetry during major hemodynamic provocations. The agreement between Capno-SvO 2 and CO-oximetry was comparable to that found for fiberoptic SvO 2 vs. CO-oximetry. Furthermore, Capno-SvO 2 demonstrated a slightly more accurate ability to detect change in SvO 2 than fiberoptic SvO 2 .

Reliability in consistency during repeated measures and the ability to generate absolute values that corresponds acceptably with the gold standard can be considered absolute prerequisites for any new monitoring technique. During stable baseline conditions, Capno-SvO 2 displayed an inherent precision matching those of both CO-oximetry and fiberoptic SvO 2 , thus, indicating a reliable monitoring system. During the following hemodynamic interventions Capno-SvO 2 generated values close to the gold standard method and the overall agreement between Capno-SvO 2 and CO-oximetry was within the predefined 95% limits of agreement of 15% points and well below the a priori determined limit for a PE of < 30%. There was an overall tendency for Capno-SvO 2 to display slightly higher SvO 2 values compared to CO-oximetry even if this difference was relatively small and within clinically acceptable limits. Fiberoptic SvO 2 showed a smaller bias and narrower limits of agreement against CO-oximetry than that recorded for Capno-SvO 2 . Even if the difference in agreement against gold standard was relatively similar for both methods, the fact that fiberoptic SvO 2 showed slightly better agreement is not entirely surprising since this value is generated from direct estimation of SvO 2 in the actual pulmonary artery whereas the Capno-SvO 2 is a figure derived from mathematical analysis of an induced variability exhaled CO 2 . Both Capno-SvO 2 and fiberoptic SvO 2 showed variable levels of agreement against CO-oximetry depending on the type of hemodynamic intervention. During stable baseline conditions, both Capno-SvO 2 and fiberoptic SvO 2 showed near enough equal agreement against gold standard. This pattern was repeated for the FiO 2 step which is reassuring since increased FiO 2 is a common method of augmenting oxygen delivery in the clinical setting.

Differences between Capno-SvO 2 and CO-oximetry can be attributed to mainly two factors. Firstly, issues related to CO EPBF calculations i.e., disturbances in the prerequisites for the capnodynamic method, mainly the assumption of stable or slowly varying mixed venous CO 2 content and the use of updated Hb levels. Secondly the incorporated RQ value will affect the Capno-SvO 2 and thus its level of agreement against CO-oximetry.

The relatively high bias and limits of agreements seen during the fluid resuscitation (especially data points 0 and 5 min) and cava occlusion step is most likely due to initial disturbances in the mixed venous CO 2 content and Hb level.

Agreement of absolute values is central, but in the clinical context trending ability may be even more important [25] .

In this study, Capno-SvO 2 showed a very good concordance rate when compared to the gold standard, detecting 98% of the changes, which is well in line with the established fiberoptic method. In addition, the agreement between COoximetry and Capno-SvO 2 during stable baseline conditions was very good. Appropriate agreement during stable conditions in combination with a high concordance rate against CO-oximetry, makes Capno-SvO 2 potentially interesting as an early warning sign of not only more major hemodynamic deteriorations but also minor hemodynamic changes (as shown in our previous publication) [8] .

Even if the Capno-SvO 2 technique showed potentially promising performance in the current study, like most monitoring methods it has inherent limitations that needs to be considered and further investigated, particularly if applied in a clinical setting.

The fiberoptic SvO 2 method was recalibrated against COoximetry four times during the protocol to optimize its performance as shown in Fig. 1 . Normally, the fiberoptic system is intended to be calibrated once daily and not frequently recalibrated [26] . As a consequence of these frequent recalibrations, not corresponding to normal clinical routine, the subsequent fiberoptic SvO 2 values will have affected the performance of the fiberoptic catheter in a positive way. The Capno-SvO 2 was recalibrated at the same time points as the fiberoptic system but only against the current Hb level since the Capno-SvO 2 method is independent from repeated alignment against gold standard CO-oximetry obtained mixed venous saturations (as is the case for fiberoptic SvO 2 ).

The RQ value is an important determinant in estimating Capno-SvO 2 and will affect the agreement between Capno-SvO 2 and CO-oximetry. Mathematically, choosing a higher RQ will elevate the Capno-SvO 2 and vice versa. Statistically this affects accuracy, but not precision -i.e., bias will shift and will subsequently move upper and lower limit of agreements equally in parallel [14] . It will, however, not have an impact on the trending ability, maybe the most important feature of a monitoring method, as discussed above. In this study the RQ was directly measured, and the mean value of all measurements was used for calculations of Capno-SvO 2 . In the clinical setting it is more likely that RQ will be taken from tabulated values since a direct measurement is impractical with currently available methods. Furthermore, RQ depends on fasting time and the nutritional substrate given and this needs to be taken into consideration when evaluating the recorded RQ [27, 28] . In the current study, the animals were fasted and kept on a low-level glucose maintenance infusion, a common practice during anaesthesia. The scenario may have been different if nutritional status and/or infusions had been altered regarding glucose concentration or type of substrate, something that can be of importance in the intensive care setting [27] . Despite this, using the mean RQ for the whole group still resulted in acceptable agreement and trending ability.

In its current form, the Capno-SvO 2 method requires controlled mechanical ventilation [7, 29] . However, most of the patients that would benefit from continuous non-invasive assessment of SvO 2 will already be subjected to controlled mechanical ventilation both in the operating room and in the intensive care unit. Still, the fact that the method requires controlled ventilation will exclude patients that are spontaneously breathing or are treated with various modes of patient triggered ventilation.

Although Capno-SvO 2 has the potential to considerably expand the ability to continuously monitor SvO 2 compared to today, it is important to emphasize that Capno-SvO 2 is not a substitute for the proper use of a pulmonary artery catheter since it does not provide information regarding relevant pressure and resistance parameters. However, it could potentially provide real time SvO 2 monitoring in situations where a pulmonary artery catheter is neither practical or justifiable due to its invasive nature, associated risks, and cost. Thus, the potential role of Capno-SvO 2 deserves further translational studies to define its place in monitoring of patients that are cared for in the operating room or in intensive care.

In conclusion, the current study shows that the Capno-SvO 2 method is in close agreement with the gold standard CO-oximetry and displays good trending ability even during major changes in oxygen delivery. These features of the Capno-SvO 2 method, in combination with its noninvasive nature, may offer a novel real time option for SvO 2 -monitoring. Even if a pulmonary artery catheter is of seminal importance for complete hemodynamic assessment, the Capno-SvO 2 method could facilitate more advanced hemodynamic surveillance when a pulmonary artery catheter is not warranted, technically possible (such as in pediatric practice) or even contraindicated, thereby acting as a useful adjunct to more traditional hemodynamic monitoring.

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