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BACKGROUND OF THE INVENTION
The present invention is directed to an apparatus and method of its use for
determining non-invasively the concentrations of certain blood analytes.
More particularly, the invention is directed to a low cost apparatus
intended for home use by diabetics to monitor and measure blood glucose
levels.
Persons suffering from diabetes may typically monitor their own glucose
concentrations with periodic daily measurements, usually four times each
day. Present methods require the diabetic to draw a blood sample for each
test and to use a chemical reagent in the test procedure for measuring
glucose concentration. Blood extractions for such tests often become a
real burden to the diabetic and, in addition, the chemical reagents used
in the tests are quite expensive, particularly in view of the large number
of tests required. Therefore, a simple and accurate method and apparatus
for non-invasively measuring glucose concentration would be most
desirable. Further, such an apparatus which could be supplied at
relatively low cost and used by a diabetic at home, in place of present
invasive techniques, is particularly desirable.
Various kinds of apparatus and related methods for the non-invasive
determination of glucose concentrations, as well as concentrations of
other blood analytes, are known in the art. European Pat. Application No.
84840212, filed May 4, 1984 (Publication No. 0160768, dated Nov. 13, 1985)
describes such an apparatus and its method of use. The described method
uses dispersive technology in which a monochromator directs two or more
separate wave lengths of light into body tissue, either transmissively or
reflectively, for individual glucose absorbance measurements. A
microprocessor then calculates the glucose concentration from the series
of such absorbance measurements. The techniques and apparatus described in
the above identified application are typical of the traditional methods of
near infrared analysis based on the measurement of absorbance at a single
or multiple specific wavelengths.
Non-invasive, in vivo monitoring of oxidative metabolism, utilizing both
transmissive and diffuse reflective methods, is disclosed in U.S. Pat.
Nos. 4,281,645 and 4,223,680, respectively. However, both patents describe
techniques utilizing the measurement of infrared light absorbance at
specific individual wavelengths.
The concentrations of certain major blood compounds, such as glucose and
cholesterol, are much lower than concentrations of compounds typically
analyzed by near infrared spectrometry. Glucose concentration averages
only about 0.1% by weight (1000 ppm) of blood serum. Furthermore, an
accuracy of.+-.50 ppm is required for any meaningful measurement of
concentration. Thus, sensitivity to IR absorption measurements has
traditionally been a problem in determining glucose concentration. Another
problem concerns the existence of other blood serum components which
compete with glucose as light absorbers in the near infrared spectral
region where glucose is moderately or strongly absorbing. Thus,
interference from such competing components as proteins and water has
typically been a problem. In addition, the concentrations of serum
proteins are significantly higher than glucose in the spectral regions of
interest, thereby compounding the interference problem.
It is also recognized that there are practical limits on the spectral
bandwidth in the near infrared region which can be used for meaningful
glucose measurements and that reflective and transmissive measurements
cannot both be used effectively over that bandwidth. At wavelengths less
than about 900 to 1,000 nm (nanometers), other strongly absorbent
materials also exist and the specific absorption due to glucose may be too
small to provide the necessary sensitivity and accuracy, particularly in
view of the interfering absorbers. In the range of 1000 to 1800 nm,
glucose absorption is somewhat improved, but still relatively low. IR
absorbence by glucose in the range of 1800 to 2800 nm is much greater and,
at least theoretically, higher absorbance in this range should provide
sufficient sensitivity to accurately measure glucose concentrations.
However, at wavelengths greater than 1800 nm, light is strongly absorbed
by water and has little penetration capability into glucose-containing
tissue, despite the high specific absorption by glucose at these
wavelengths. As a result, transmissive measurements in the region above
about 1800 nm are impractical.
Non-dispersive correlation spectrometry, utilizing a relatively wide
infrared spectral band, has long been used in gas analysis, such as engine
gas emission analysis. A gas-filter correlation spectrometer correlates
spectral absorption signals from the gas being measured and a gas in a
filter. In particular, systems utilizing a so-called "negative filter"
have been found to be particularly effective and exhibit a low sensitivity
to interfering gases. One such system is described in Cha and Gabele,
"Study on Infrared Gas-Filter Correlation Spectrometer for Measuring
Low-Concentration Methanol Gases", Optical Engineering, Volume 25, No. 12,
pages 1299-1303 (December 1986). However, gas filters used in gas
correlation cells are relatively easy to make and use. A gas correlation
cell typically comprises a sealed glass or plastic cell that contains the
gas of interest at a predetermined concentration. A liquid correlation
cell, on the other hand, is much more difficult to design, make and use
and, to applicant's knowledge, the principles of gas filter correlation
spectrometry have not been applied to liquid analysis.
There is a particular need today for a non-invasive instrument which could
be used by the diabetic at home for measuring and monitoring glucose
levels. Such a device would eliminate the need for chemical tests
requiring expensive reagents, as well as the burden and trauma associated
with multiple daily blood sampling. The device should also be relatively
low in cost and, ideally, be less than the annual cost of current invasive
methods.
SUMMARY OF THE INVENTION
The present invention is directed broadly to an apparatus and related
method for the non-invasive measurement of blood analyte concentration
utilizing non-dispersive near infrared correlation spectrometry. The
apparatus and method are particularly adaptable to the measurement of
glucose concentration, but may be applied to measuring the concentration
of a number of blood analytes. The apparatus and method are adapted to
utilize either transmissive or diffuse reflective measurements.
A source of modulated light in the near infrared bandwidth is transmitted
to a source containing the blood analyte. The light is either reflectively
or transmissively modified by the source and the spectrally-modified light
is retransmitted to a beam splitter to provide two beams for the
correlation analysis. One beam is directed to a correlation cell which
functions as a negative optical filter by providing an absorption spectra
for the analyte at a level sufficient to block light over the selected
bandwidth for the expected concentration range of the analyte. The other
beam is directed to a reference cell, in the form of a neutral density
filter, which has an absorption spectra sufficient to block light equally
at all wavelengths in the selected bandwidth. The intensities of each of
the beams are measured by a photosensor and a signal representative of the
difference in the beam intensities, which is proportional to the analyte
concentration, is generated and converted into a direct indication of
analyte concentration.
In the preferred embodiment of the apparatus, for measuring glucose
concentration, a non-dispersed band of near infrared light is transmitted
via a fiber optic link to the skin surface of the tissue to be analyzed.
The light is directed to be diffusely reflected from the skin surface and
the spectrally-modified light is divided by a beam splitter. The negative
correlation filter comprises glucose in a non-absorbing solvent or a
coating of glucose solution on a glass substrate.
Utilizing diffusely reflective measurement allows operation in a selected
bandwidth where glucose absorbance is much higher (in the range of above
about 1800 nm). Necessary sensitivity for accurate glucose measurement
exists in this range, and sensitivity is substantially improved with
non-dispersive techniques in which IR absorbance information over the
entire bandwidth may be used.
BRIEF DESCRIPTION OF THE DRAWING
FIG. 1 is a schematic representation of the apparatus of the preferred
embodiment of the present invention.
FIG. 2 is a schematic representation of an alternate embodiment of the
invention.
DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT
An apparatus for the non-invasive infrared analysis of blood chemistry is
shown in FIG. 1. It will be hereinafter described with respect to
construction and use in its preferred embodiment for the measurement of
glucose concentration. A spectrometer 1 includes a light source in the
form of a tungsten halogen lamp 10 which generates a spectrum of light in
the visible and near infrared regions. The light from the lamp 10 is first
modulated by passing it through a chopper wheel 11 to provide light
signals which can be processed to minimize background noise resulting from
ambient light and other stray signals. The light is then focused by a lens
12 into a fiber optic transmission cable 13 where it is directed to the
source of the analyte, i.e. glucose, to be measured. As shown in FIG. 1,
the glucose source is blood within the tissue of an ear lobe 14.
The light carried in the fiber cable 13 may be transmitted through the ear
lobe 14 or it may be caused to impinge on the skin surface of the tissue
(such as a patient's arm) at an angle where it is absorbed by tissue
material near the surface and reflected as diffuse radiation. In either
case, the light is spectrally-modified as a result of infrared absorption
by the blood and tissue components, including glucose. In the apparatus
shown, an optrode 15 at the end of the fiber cable 13 transmits light
energy to the skin surface, receives the spectrallymodified light
transmitted through the tissue, and retransmits it into the reception
fiber optic cable 16. The spectrally-modified light is then returned to
the spectrometer 1 through a pair of lenses 17 separated by a slit 18
which aids in rejecting stray light.
In the embodiment utilizing diffuse reflectances, a near infrared bandwidth
in the range of 1800 to 3400 nm is preferred. Glucose is known to be much
more strongly absorbing in this range but, because of the similar high
absorbance by water in this region, transmissive measurements are not
practical. Serum proteins, which exist in signficantly higher
concentrations than glucose in the near infrared spectral regions of
interest, constitute a serious source of interference, particularly when
measuring transmissively. However, human skin layers act as a natural
filter that allow smaller glucose molecules to move to the surface, but
restrict movement thereto of the larger protein molecules. Therefore,
reflective skin surface measurements are less subject to protein
interference than are transmissive measurements. Furthermore, a
correlation between skin surface glucose and serum glucose has been
established and direct measurement of the former can be converted into the
latter.
The light exiting lens 17 is directed through a beam splitter 19. One of
the modified light beams from the splitter is directed through a
correlation cell 20 comprising a negative correlation filter 21. The
correlation filter contains a glucose absorption spectra sufficient to
block light for the maximum anticipated concentration of glucose in the
tissue sample. The correlation filter may comprise an aqueous solution of
glucose at a predetermined concentration. Such water solutions are
preferred because they simulate blood absorption. However, water solutions
of glucose are often unstable. The negative correlation filter 21 may also
comprise a non-aqueous glucose solution, using a non-absorbing solvent.
Alternatively, the filter may comprise a coating of a glucose solution on
a glass substrate. In the two latter cases, a separate layer of water is
also used to simulate water absorption in the blood.
The other modified split beam is directed through a reference cell 22
which, in the preferred embodiment, comprises a neutral density optical
filter 23. The neutral density filter 23 is a standard device made with a
broad flat absorption spectrum sufficient to block light equally at all
wavelengths in the infrared range of interest.
In operation, as the level of glucose changes, the light passing through
the negative correlation filter 21 remains unaffected because it has
already blocked all light in the glucose absorption bands. The intensity
of the light passing through the neutral density filter 23 of the
reference cell 22, on the other hand, will be reduced in proportion to
glucose concentration. The difference in light intensity between the beams
exiting the respective filters 21 and 23 is a measure of glucose
concentration.
The intensities of the beams exiting the negative correlation filter 21 and
neutral density filter 23 are measured, respectively, by photosensors 24
and 25. For the infrared bandwidth indicated above, a lead sulfide
photodetector is preferred. The photosensors convert the measured light
into signals representative of the light intensities, which signals are
fed to a lock-in amplifier 26 which generates a signal representative of
the difference in the measured intensities of the two beams. The
differential signal is converted to digital form for input into a
microprocessor 27 to calculate the actual glucose concentration. The
concentration may be conveniently indicated by a suitable digital display
28. It should be noted that the modified light beams exiting the filters
21 and 23 could be directed to and utilize a single photosensor. This
would help eliminate or reduce errors in drift.
When utilizing reflective measurements at longer wavelengths (in the range
of 2700 to 3400 nm for glucose analysis, sensitivity may be substantially
enhanced because of the stronger absorbance by glucose in this range.
However, conventional optical fibers are not suitable for infrared
transmission at these wavelengths and more expensive and fragile fibers,
such as fluoride-based, are required. An alternate construction,
eliminating the use of fiber optics, comprises a hand-held optical head
which contains the light source, filters and photodectors.
Although the foregoing device and its method of operation were described
with respect to the measurement of glucose concentration, other blood
analytes such as cholesterol, triglycerides and uric acid may be similarly
measured.
In FIG. 2, there is shown an alternate arrangement of an apparatus for the
transmissive in vitro measurement of blood analytes. The basic principles
of operation and analysis are the same as the apparatus for in vivo
measuremnt using diffuse reflective or transmissive light in the preferred
embodiment of FIG. 1, but with a few differences which will be discussed
hereinafter.
A light source, such as a quartz halogen lamp 30, generates light in the
near infrared range which, after passing through a diffuser 31, is
directed transmissively through a sample 32 of human blood serum. Whole
blood samples may also be used, but the instrument must be adjusted for
higher light intensity and amplifier gain to penetrate the higher density
whole blood. The serum (or blood) sample may be held in a conventional
cuvette. Light exiting the serum sample 32 is passed through a slit 33 to
eliminate stray light signals. For glucose measurement, the bandwidth
should preferably range from 900 nm on the shorter wavelength end, where
glucose absorbance becomes relatively higher, to about 1800 nm on the
longer wavelength end, above which transmissive measurements are
impractical due to the high absorbance by water.
The spectrally-modified light, as a result of its passage through the serum
sample 32, is collimated by passage through lens 34 and directed into a
beam splitter 19. The beam splitter 19, cells 20 and 22, photosensors 24
and 25, and the electronics for modifying the signals and computing the
concentrations may be the same as in the preferred embodiment of FIG. 1.
However, as previously suggested with respect to the description of the
preferred embodiment, a single photosensor 35 may be substituted for the
dual photosensors 24 and 25. With a single photosensor 35, the light paths
from the cells 20 and 22 will have to be appropriately altered, as
indicated. Furthermore, in order to provide the capability to discriminate
between and separate the two light beams directed to the photosensor 35
and the signals produced thereby, the beam splitter 19 may be replaced
with a mirror/chopper device (not shown) which would alternately direct
the light from the sample to the correlation cell 20 and the reference
cell 22. Alternatively, shutters could be interposed in the paths from the
beam splitter for the same purpose.
The procedures for balancing either of the apparatus shown in FIG. 1 or
FIG. 2, prior to making a measurement, are the same. In the in vivo
version shown in FIG. 1, a reference cell 22 is positioned in the light
path 13 in place of the ear 14. For the in vitro version shown in FIG. 2,
a reference cell 22 is substituted for the sample cell 32. And, in either
case, the output of the correlation cell channel is adjusted to provide a
zero output from the amplifier 26. Next, a correlation cell 20 is
substituted for the reference cell in the position of the ear 14 or sample
32, depending on the apparatus, and the output of the amplifier 26 is set
at the glucose concentration value of the correlation cell. The apparatus
is now balanced and ready for use. Although the water layers used with the
reference and correlation cells have less absorbance than whole blood or
blood serum, this difference in absorbance affects both channels equally
and cancels out. Thus, when actual samples are run, the only difference in
the output of the two channels will be as a result of the glucose in the
sample.
For the analysis of blood analytes other than glucose, an appropriate
negative correlation filter would have to be substituted. As in the case
of glucose measurement, the substitute filter requires an absorption
spectra for the analyte to be measured which is sufficient to block light
in the selected bandwidth for the maximum expected concentration of that
analyte.
In lieu of a neutral density filter 23, in either of the foregoing
embodiments, the reference cell 22 may comprise a compensator cell having
a spectrum equivalent to a high level of all of the encountered
interference. A compensator cell would respond only to changes in the
analyte of interest and not to changes in the interferring substances. An
alternate approach to compensating for interferring analytes utilizes an
interference cell ahead of the sample source, e.g. serum sample 32 in FIG.
2. Like a compensator cell, an interference cell would contain the spectra
of the potentially interfering substances sufficient to block light in the
interfering absorption bands.
The correlation techniques useful in determining the concentration of
glucose or other blood serum analytes described herein provide significant
advantages over prior art methods of near infrared analysis based on
measurement of absorbance at single or multiple specific wavelengths. The
method and apparatus described use information over the entire bandwidth
of interest and are limited only by the bandwidth of the photosensor. This
substantially enhances the sensitivity of the instrument. An equally
important advantage of the disclosed correlation technique is its
insensitivity to changes in overall infrared absorbance caused by factors
which are unrelated to concentration of the analyte being measured.
Varying skin and other tissue characteristics can produce significant
variations in the overall near infrared absorbance levels. However, in the
disclosed method, these variations are not significant because they cancel
out in differencing the signals from the correlation cell and reference
cell.
Various modes of carrying out the invention are contemplated as being
within the scope of the following claims particularly pointing out and
distinctly claiming the subject matter which is regarded as the Invention.
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