Method and Device for Determining the Glucose Concentration in Tissue Liquid

Information

  • Patent Application
  • 20080153118
  • Publication Number
    20080153118
  • Date Filed
    November 07, 2007
    17 years ago
  • Date Published
    June 26, 2008
    16 years ago
Abstract
The invention relates to a method and a device for determining the glucose concentration in tissue fluid whereby test values for glucose and for an endogenous reference substance are detected in a sample liquid obtained by microdialysis, microperfusion or ultrafiltration, and the glucose value is corrected in accordance with the test value for the reference substance. The recovery rate for glucose is determined from a non-linear relationship with the recovery rate for the ionic reference substance, and the test value for glucose is corrected therewith. In addition, the concentration of lactate and/or pyruvate is used as a further reference substance in the sample liquid to make further corrections.
Description
BACKGROUND

1. Field of the Invention


The invention concerns a method for determining the glucose concentration in tissue fluid in which test values for glucose and for an endogenous reference substance are detected in a sample liquid obtained from a body tissue by microdialysis, microperfusion or ultrafiltration and the test value for glucose is corrected in accordance with the test value for the reference substance. The invention also concerns a corresponding device.


2. Description of the Prior Art


Body tissue consisting of cells in a liquid environment in which metabolic products are transported between the cells and the blood vessels. In order to monitor glucose of diabetic patients, for example, it is possible to insert a probe into tissue for long periods in order to continuously obtain components from the tissue fluid by means of diffusion processes and to determine the glucose content in the tissue from the effusate. This can correlate closely with the blood glucose content without requiring an invasive access to the blood circulation. The measurement can take place outside of the body in which case the sample liquid is applied to a sensor. In this connection an ionic reference technique is known in which an ionic reference value and in particular Na+ is detected simultaneously with glucose by an ion-selective electrode in order to calibrate the recovery of the glucose in the dialysate. In this case, it is assumed that the known concentration of the reference substance in the body fluid is substantially invariant. A prerequisite of the known evaluation methods is that there is a strict linear relationship between the recovery of the endogenous calibrator and glucose in the sample liquid. However, empirical comparative measurements make this seem doubtful.


SUMMARY OF THE INVENTION

The invention considers local effects in the tissue as well as transport resistances which occur due to the special probes that are used for microdialysis, microperfusion or ultrafiltration. Accordingly, in embodiments of the invention, the concentration of lactate and/or pyruvate as a reference substance is determined in the sample liquid. This enables the specific metabolic paths of glucose degradation to be utilized in order to draw conclusions about effects on the measurement correction that are due to local tissue reactions.


A concentration ratio of lactate to pyruvate in the sample liquid is advantageously determined to correct the test value for glucose. In embodiments of the invention, at a concentration ratio of lactate to pyruvate in a selected middle range of between about 10:1 and about 20:1, a linear correction dependent on the concentration ratio is carried out, and in a higher range above the selected range and above a concentration ratio of 20:1 the test value for glucose is corrected by a constant. An analogous correction is also conceivable when using lactate alone as the reference substance.


In embodiments of the invention, the recovery rate (RGLU) for glucose is determined from a non-linear relationship with the recovery rate (RREF) for the ionic reference substance, and the test value for glucose is corrected therewith. In this manner it is possible to carry out a type of technical correction in a specifically adapted form for effects that are caused mainly by the specific probe technology, for example, due to the membrane processes. This allows for an accurate correction. This may be due to the fact that the recovery of the ion reference is higher than that of glucose due to the small particle size and/or due to the charge, as may be the case with rapid perfusion. Hence the non-linear compensation curve runs in a curve shape below the bisecting line.


According to embodiments of the invention, the recovery rate (RGLU) for glucose is determined according to the relationship





1-RREF=(1-RGLU)k


in which k is a predetermined value. In this connection, the value k can be determined empirically as the ratio of resistances for the transfer of glucose and the reference substance between tissue fluid and sample liquid. Furthermore, it is proposed that the recovery rate (RREF) for the reference substance is determined as the ratio of the test value for the reference substance in the sample liquid and a constant concentration value in the tissue fluid. Sodium is advantageously used as an endogenous ionic reference substance.


A particularly effective and accurate compensation can be achieved by using sodium as a reference substance for a correction of deviations due to the measurement technology and lactate and/or pyruvate as a reference substance for a correction of locally-related deviations of the test value for glucose in the sample liquid from the actual glucose concentration in the tissue of the organism.


The compensation described above can be used particularly advantageously in procedures in which a probe located in the tissue is used to obtain sample liquid by perfusion with rinsing liquid or by applying a negative pressure.


An additional functionality is achieved by means of the fact that a malfunction is signalized when an upper and/or lower predetermined threshold of the test value for the reference substance is exceeded.


The above-mentioned process may be achieved utilizing a corresponding device for carrying out the process. Accordingly a sensor unit is provided for a device where said sensor unit is designed to determine the concentration of lactate and/or pyruvate as a reference substance in the sample liquid.


In embodiments of the invention, the evaluation unit has an evaluation program which determines the recovery rate (RGLU) for glucose from a non-linear relationship with the recovery rate (RREF) for the ionic reference substance, and the test value for glucose is corrected therewith.





BRIEF DESCRIPTION OF THE DRAWINGS

The above-mentioned and other features of this invention and the manner of obtaining them will become more apparent and the invention itself will be better understood by reference to the following description of an embodiment of the present invention taken in conjunction with the accompanying drawings, wherein:



FIG. 1 shows a block diagram of a measuring arrangement for determining glucose;



FIG. 2 shows a schematic representation of a microdialysis system as a measuring arrangement;



FIG. 3 shows a probe of a microdialysis system according to FIG. 2 in a partially enlarged view;



FIG. 4 shows a greatly simplified reaction scheme of glucose processing in body cells;



FIG. 5 and FIG. 6 show empirical measurement data of microdialysis examinations using lactate/pyruvate compensation curves;



FIG. 7 shows a measurement diagram corresponding to FIG. 5 for an examination by means of ultrafiltration; and



FIG. 8 shows a measurement diagram of the glucose and sodium recovery by means of microdialysis using a calculated compensation curve.





Although the drawings represent embodiments of various features and components according to the present invention, the drawings are not necessarily to scale and certain features may be exaggerated in order to better illustrate and explain the present invention. The exemplification set out herein illustrates embodiments of the invention, and such exemplifications are not to be construed as limiting the scope of the invention in any manner.


DETAILED DESCRIPTION OF EMBODIMENTS OF THE INVENTION

For the purposes of promoting an understanding of the principles of the invention, reference will now be made to the embodiments illustrated in the drawings, which are described below. It will nevertheless be understood that no limitation of the scope of the invention is thereby intended. The invention includes any alterations and further modifications in the illustrated device and described methods and further applications of the principles of the invention, which would normally occur to one skilled in the art to which the invention relates. Moreover, the embodiments were selected for description to enable one of ordinary skill in the art to practice the invention.


The measurement arrangement according to FIG. 1 includes a probe 10 that can be inserted into subcutaneous tissue for obtaining a sample liquid, a sensor system 12 for detecting components in the sample liquid, an evaluation and control unit 14 for processing the sensor signals and controlling the measurement process as well as optionally an output unit 16 and an interface 18 to display or transmit the measured results. The probe 10 can be loaded in a known manner with perfusion fluid (microdialysis, microperfusion) or be placed under negative pressure (ultrafiltration) in order to collect the sample liquid.



FIG. 2 illustrates in more detail a microdialysis system for continuous sample collection and measurement data recording. The microdialysis probe 10 has a double-lumen membrane catheter 22 which is located in the tissue 20. The catheter 22 can be rinsed with a perfusion liquid 28 from a liquid reservoir 26 via a feed line 24. The perfusion liquid 28 may comprise any suitable solution, such as physiological saline, for example. The return line 30 of the dialysis probe 10 runs through a peristaltic or roller dosage pump 32 to a collecting vessel 34. A flow measuring cell 36 of the probe 10 may be arranged extracorporeally in the return line 30. The measuring cell 36 detects the concentration of the sought-after analyte in the dialysate, such as glucose, for example, and a reference or control substance, for example, by means of an electrochemical measurement.


The mode of operation of the microdialysis probe 10 can be seen in more detail in FIG. 3. The distal end of the catheter 22 has a dialysis membrane 38 which is embedded in the tissue 20 such that the perfusate flowing in through the inlet channel 24 is loaded through the semi-permeable membrane with constituents 40 from the intercellular tissue. The porosity of the membrane 38 is dimensioned so that the metabolic products to be measured, such as glucose, lactate and pyruvate, for example, can pass into the perfusate almost without resistance, and larger molecules are held back. Suitable alternatives may be utilized, such as microperfusion, for example. In the case of microperfusion, there may be no membrane, and the inner space of the probe 10 may be directly coupled to the tissue via perforations in the wall. In both cases the collected sample liquid 42 is aspirated through the mouth of the return channel 30, which is proximally set back from the outlet opening of the line 24.


However, due to various circumstances and in particular to local changes and transport resistances and perfusion rates, the glucose concentration in the dialysate or effusate is not equal to that of the glucose content in the tissue fluid. In order to remedy this situation the sensor unit 10, together with the evaluation unit 14, is designed to additionally determine the concentration of an endogenous reference or control substance in order to carry out a compensation for effects which falsify the measurement. Generally, the glucose concentration in capillary blood is regarded as a “gold standard” which can be determined by spot measurements using known tests.


One aspect concerns the correction of the test value for glucose on the basis of the concentration ratio of lactate to pyruvate in the sample liquid. The background to this is glucose processing in the tissue cells is illustrated in a greatly simplified manner in FIG. 4. Glucose is degraded by glycolysis to pyruvate which can in turn be utilized in an aerobic process with a high energy yield in which the largest possible number of H atoms (in the form of NADH/H+ and FADH2) are obtained which react with oxygen to form water and ATP (citrate cycle). Under anaerobic conditions pyruvate is degraded to lactate in a competing metabolic pathway. This process generates less energy so that the cells have to locally process more glucose to cover their energy requirements. The compensation method, which is elucidated in more detail in the following, is based on the idea that when lactate increases, an exceptional case is present which indicates that the general glucose concentration in the body is higher than the local concentration in the probe environment. Such local changes could, for example, result from the insertion of the probe, or from probe movements, in the tissue.



FIG. 5 shows a measurement diagram in conjunction with an embodiment of a proposed compensation curve. The deviation or difference of the glucose values measured in parallel for sample liquid and blood is plotted against the ratio of lactate to pyruvate in the sample liquid. The aim of the compensation is to reduce the deviation compared to the values in blood. For this purpose, a correction calculation is performed in the evaluation unit which is such that a linear correction is carried out at a concentration ratio of lactate/pyruvate between about 10:1 and about 20:1 (curve section 44) and that the test value for glucose is corrected by a constant above a concentration ratio of about 20:1 (curve section 46). This constant results directly from FIG. 5 by the amount for the abscissa value for section 46.



FIG. 6 shows a measurement diagram in conjunction with an embodiment of a proposed compensation curve when only lactate is used as a reference substance. The deviation or difference of the glucose values measured in parallel for sample liquid and blood is plotted against the lactate content in the sample liquid. In order to reduce the deviation compared to the values in blood, a linear correction is carried out at a lactate content between about 1.3 and about 2.5 millimoles per liter whereas the test value for glucose is corrected by a constant when the values of the lactate content are higher than this range. The constant results from FIG. 6 by the amount of the abscissa value of the line of best fit in the upper range.


With reference again to FIG. 1, in ultrafiltration a negative pressure may be applied to a membrane probe 10 by means of a suction pump or suction syringe without feeding in perfusion liquid. As a result, interstitial tissue fluid enters the suction line and is transported to a sensor 12. The semi-permeable membrane of the catheter generally only allows relatively small molecules to diffuse through together with the liquid and thus form a sample liquid which is separate from the tissue fluid. In this case, reactions due to injury can occur in the tissue which result in local changes in the glucose concentration and can be corrected by means of lactate/pyruvate measurements in the sample liquid.



FIG. 7 shows test values obtained by ultrafiltration in which the difference between the detected glucose value in the sample liquid and comparative measurements in blood is plotted as the ordinate against the ratio of lactate to pyruvate. The dashed correction curve 48 corresponds to the compensation elucidated above in connection with FIG. 5. It is also possible to only carry out a linear correction corresponding to the continuous line 50 for example in a concentration range between about 10:1 and about 30:1 lactate/pyruvate wherein the slope of the compensation curve was obtained by a fit to the test values.


According to an embodiment of the invention, test values for ions that are kept very constant in the tissue, such as Na+ ions, for example, are detected as an endogenous ionic reference substance, in addition to the glucose values in the sample liquid. In this case, it is assumed that Na+ in the tissue fluid remains substantially constant independently of the glucose processing and that a simultaneous measurement of glucose and sodium ions in the sample liquid can thus be used to deduce the transport or flow resistances in the sample collection. In the example, the recovery rate is defined as the concentration ratio of the respective substance in the tissue fluid and sample liquid. With reference to FIG. 1, the evaluation unit 14 has an evaluation routine 52 for the ionic reference correction which determines the recovery rate RGLU for glucose from a non-linear relationship with the recovery rate RREF for the ionic reference substance (Na+) and thus corrects the test value for glucose.


In particular the evaluation program 52 determines the recovery rate RGLU for glucose from the relationship





1-RREF=(1-RGLU)k   (1)


in which k is a predetermined value.


The recovery rate RREF for the reference substance is determined as a ratio from the test value for the reference substance in the sample liquid and a known constant concentration value in the tissue fluid.


The equation (1) is based on a non-linear model for recovery:









recovery
=

1
-

exp
[

-

1

Q
·

W
tot




]






(
2
)







in which Q denotes the flow rate of perfusion and Wtot denotes the total resistance as a function of the transport resistances of dialysate, membrane and tissue.


From equation (2) it firstly follows that:










1

1


n


(

1
-
recovery

)




=

-

QW
tot






(
3
)







i.e. a logarithmic transformation results in a linear dependence on the flow rate.


A factor k is now sought after which characterizes the ratio of the total resistances for glucose and sodium for a certain dialysis membrane:






W
tot(glucose)=k Wtot(sodium).


This factor k can be estimated with the aid of in vivo studies and in vitro data from equation (3) by forming the quotient.


The factor k is a function of the resistances i.e. in practice a function of the flow rate, membrane and interstitium properties:






k
=




W
tot



(
glu
)




W
tot



(
Na
)



=


1






n


(

1
-

recovery


(
Na
)



)




1






n


(

1
-

recovery


(
Glu
)



)









In vivo studies have shown that the influence of the membrane and the physiological environment (determined by osmotic effects) can also be modeled and enables an additional correction of the recovery.


If k is known, then the relationship between recovery (glucose) and recovery (sodium) can be derived from equation (2) as follows:













1
-

recovery


(
Na
)



=

exp


[

-

1


QW
tot



(
Na
)




]








=

exp


[

-

k


QW
tot



(
Glu
)




]








=


exp


[

-

1


QW
tot



(
Glu
)




]


k







=


[

1
-

recovery


(
Glu
)



]

k








(
1
)








FIG. 8 shows a diagram of the test values of the glucose recovery rate plotted against the Na+ recovery rate. In addition a proportional relationship between the recovery rates, represented by the line 54, and the compensation curve 56 according to the first equation set forth above, is shown in the diagram. It can be clearly seen that the proportional or linear relationship according to line 54 is not confirmed by the test values whereas the compensation curve 56 runs positively curved completely below the bisecting line and thus correctly describes the empirical measurements.


Thus, the compensation curve 56 can compensate for a variation in the recovery by also appropriately correcting the value for glucose on the basis of a changing Na+ recovery. In order to take into account different flow rates, the compensation curve 56 could be compressed by an additional factor which thus takes into consideration the fact that a 100% recovery cannot be reached due to the high throughput.


Any suitable substance, such as Na+, for example, may be utilized as a reference substance to correct for metrological substance. Any suitable substance, such as lactate/pyruvate, for example, may be utilized as a reference substance to correct for locally-related deviations of the test value for glucose in the sample liquid from the actual glucose concentration in the tissue.


In embodiments, the signaling of a malfunction of the measuring arrangement by a signal transmitter when a threshold value of the test value for the reference substance is exceeded may be included in the probe 10.


While this invention has been described as having an exemplary design, the present invention may be further modified within the spirit and scope of this disclosure. The application is intended, therefore, to cover any variations, uses, or adaptations of the invention using its general principles. Further, this application is intended to cover such departures from the present disclosure as come within known or customary practice in the art to which this invention pertains.

Claims
  • 1. A method for determining the glucose concentration in a tissue fluid comprising the steps of: measuring an uncorrected glucose concentration in the tissue fluid;measuring a concentration of at least one reference substance and glucose in a sample liquid;determining a corrected glucose concentration in the tissue fluid based upon the measured concentration of the at least one reference substance and glucose in the sample liquid.
  • 2. The method as set forth in claim 1 wherein the at least one reference substance includes lactate or pyruvate.
  • 3. The method as set forth in claim 1 wherein the at least one reference substance includes lactate and pyruvate.
  • 4. The method as set forth in claim 3 further including the step of determining a concentration ratio of lactate to pyruvate in the sample liquid in order to correct the test value for glucose.
  • 5. The method as set forth in claim 4 further including the step of utilizing a linear correction factor to determine the corrected glucose concentration in the tissue fluid if the concentration ratio of lactate to pyruvate generally falls within the range between about 10:1 to about 20:1.
  • 6. The method as set forth in claim 4 further including the step of utilizing a constant to determine the corrected glucose concentration in the tissue fluid if the concentration ration of lactate to pyruvate is generally about 20:1.
  • 7. The method as set forth in claim 1 wherein the uncorrected glucose concentration is measured by a technique selected form the group consisting of microdialysis, microperfusion or ultrafiltration.
  • 8. A method of determining a glucose concentration in a tissue fluid comprising the steps of: measuring an uncorrected concentration of glucose in the tissue fluid;measuring a concentration of glucose in a sample liquid;measuring at least one reference substance in the sample liquid;determining a recovery rate for glucose (RGLU) determined from a recovery rate for the reference substance (RREF); anddetermining a corrected concentration of glucose from the recovery rate for glucose.
  • 9. The method as set forth in claim 8 wherein the recovery rate for glucose is determined according to the equation 1-RREF=(1-RGLU)k and k is a predetermined value.
  • 10. The method as set forth in claim 9 further including the step of determining a value for k based upon a ratio of the resistances for the transfer of glucose and the reference substance between the tissue fluid and the sample liquid.
  • 11. The method as set forth in claim 10 further including the step of calculating the recovery rate for the reference substance based upon the ratio of a tested value of the reference substance in the sample liquid and the constant concentration value in the tissue fluid.
  • 12. The method as set forth in claim 7 wherein the reference substance is an ion of sodium.
  • 13. The method as set forth in claim 7 wherein the reference substance is lactate.
  • 14. The method as set forth in claim 7 wherein the reference substance is pyruvate.
  • 15. The method as set forth in claim 7 wherein the measuring steps are conducted ex vivo.
  • 16. The method as set forth in claim 7 further including the steps of: inserting a probe into the tissue; andobtaining the sample liquid using the probe.
  • 17. The method as set forth in claim 16 wherein the probe obtains the sample liquid using negative pressure.
  • 18. The method as set forth in claim 7 further including the step of signaling a malfunction when a measured test value falls outside a predetermined range.
  • 19. A device for determining the glucose concentration in a tissue fluid including: a sensor unit configured to measure a plurality of concentration values for glucose and a reference substance in a sample liquid; andan evaluation unit configured to correct the concentration value for the glucose according to the concentration value for the reference substance;wherein the reference substance consists of at least one of lactate and pyruvate.
  • 20. The device as set forth in claim 19 wherein the evaluation unit calculates the concentration ratio of lactate to pyruvate in the sample liquid.
  • 21. The device as set forth in claim 20 wherein the evaluation unit carries out a linear correction of the glucose content when the concentration of lactate to pyruvate falls within a prescribed range.
  • 22. The device as set forth in claim 21 wherein the evaluation unit corrects the glucose content based upon a constant when the concentration of lactate to pyruvate exceeds the prescribed range.
  • 23. The device as set forth in claim 19 wherein the evaluation unit determines the recovery rate of glucose (RGLU) from a non-linear relationship with the recovery rate for an ionic reference substance (RREF) and calculates the corrected glucose concentration.
  • 24. The device as set forth in claim 19 further including a signal capable of indicating a malfunction when a measured value for the test substance falls outside a predetermined range.
Priority Claims (1)
Number Date Country Kind
05009986.0 May 2005 EP regional
Continuations (1)
Number Date Country
Parent PCT/EP2006/004179 May 2006 US
Child 11936569 US