Patent Grant
7678567
1. Field of the Invention
The present invention relates to an apparatus for measuring a specific molecule included in a specimen and in particular to an optical biosensor.
2. Description of the Related Art
A planar lightwave circuit sensor using optical waveguide phenomenon is widely spread as the sensor to measure the amount of the bio molecules existing in body fluid such as blood. As shown in
An existing method for analyzing the bio molecules existing in the blood by the planar lightwave circuit sensor is as follows. At first, the blood is collected from vein with a syringe. The collected blood is dropped on the GOD membrane 5. The laser light is emitted from the light source 6 and diffracted by the first grating 3. The diffracted light penetrates the optical waveguide membrane 2. The evanescent wave is generated at the interface between the optical waveguide membrane 2 and the GOD membrane 5. The intensity of the evanescent wave changes by reaction between the dropped bio molecules contained in the blood and the GOD. The photo detector 7 receives the diffracted light from the second grating 4 and detects the changes of the evanescent wave intensity to analyze the bio molecules contained in the blood as disclosed in Japanese Patent Application Hei9-61346.
However, manufacturing the evanescent wave generates requires precision apparatus and techniques. This is because the incident light reaching at the interface should be diffracted at appropriate angle to measure the change of the evanescent wave intensity precisely.
An aspect of present invention inheres in an optical biosensor having a total reflection plate so as to totally internally reflect and transmit an incident light, a first grating and a second grating disposed separately on the total reflection plate, and a sensing membrane that is containing an enzyme and a chromogenic reagent and is sandwiched by the first and second gratings on the total reflection plate.
Various embodiments of the present invention will be described with reference to the accompanying drawings. It is to be noted that the same or similar reference numerals are applied to the same or similar parts and elements throughout the drawings, and the description of the same or similar parts and elements will be omitted or simplified.
With reference now to
The total reflection plate 10 is composed of quartz (SiO2), for example. The first and second gratings 11a, 11b are composed of material of which refractive index is higher than the total reflection plate 10. For instance, titanium oxide (TiO2), zinc oxide (ZnO), niobic acid lithium (LiNbO3), gallium arsenide (GaAs), indium tin oxide (ITO), polyimide, or tantalum oxide (Ta2O5) is deposited on the total reflection plate 10 by chemical vapor deposition (CVD) and selectively etched away with dry etching to form the first and second gratings 11a, 11b.
The sensing membrane 12 is formed by gelation of the enzyme and the chromogenic reagent with cellulose derivative. For example, glucose oxidase (GOD), peroxidase (POD), or mutarotase is useful as the enzyme in the sensing membrane 12 when the biosensor is used for inspecting glucose in a body fluid. 3,3′,5,5′-tetramethylbenzidine (TMBZ) is useful for the chromogenic reagent, for example. Reaction formulas (1)-(3) show reactions between the glucose and the enzyme to stain the sensing membrane 12. It should be noted only product related to pigmentation of the sensing membrane 12 is shown in each of reaction formulas (1)-(3).
Glucose+GOD→H2O2 (1)
H2O2+POD→Oxygen Radical (O*) (2)
O*+Chromogenic reagent→Pigmentation (3)
The protection sheet 13 is composed of material of which refractive index is lower than the first and second gratings 11a, 11b. Also, it is desirable to use the low refractive index material that does not react with the reagents such as the enzyme and the chromogenic reagent. Coating such low refractive index material on the total reflection plate 10 forms the protection sheet 13.
With reference again to
When the incident light is refracted at the interface between the total reflection plate 10 and the sensing membrane 12, evanescent wave is absorbed by the pigmentation of the sensing membrane 12. The pigmentation intensity and the absorbed light intensity are in proportion. Also, the pigmentation intensity and the amount of specimen such as the glucose dropped on the sensing membrane 12 are in proportion.
The incident light reaches the second grating 11b and the incident light is diffracted in the direction of a photo detector 22. By detecting the difference between the light intensities emitted by the light source 21 and received by the photo detector 22, it becomes possible to calculate the amount of specimen such as the glucose dropped on the sensing membrane 12.
The optical biosensor in accordance with the embodiment of the present invention employs simplified structure. Therefore, it is possible to manufacture the optical biosensor easily.
(FIRST MODIFICATION)
With reference now to
Since the quartz is expensive material, the optical biosensor shown in
The glass plate 10a is composed of non-alkali glass, for example. The silicon oxide layer 10b is formed by depositing silicon oxide (SiO2) on the glass plate 10a by the CVD or the spattering process. Without the silicon oxide layer 10b, heterogeneous metals exist on the glass plate 10a. Therefore, if the sensing membrane 12 is disposed on the glass plate 10a directly, such heterogeneous metals affect preciseness of the inspection.
As shown in
(SECOND MODIFICATION)
With reference now to
Since the quartz is expensive material as described in the first modification, the optical biosensor shown in
The glass plate 10a is composed of non-alkali glass, for example. The titanium oxide layer 10c is formed by depositing titanium oxide (TiO2) on the glass plate 10a by the CVD or the spattering process. The titanium oxide layer 10c has thickness of 180 nm-200 nm, desirably 200 nm so as to maximize the absorbance of the incident light at the interface between the titanium oxide layer 10c and the sensing membrane 12.
After the titanium oxide layer 10c is formed, it is possible to delineate the first and second gratings 11a, 11b easily by selectively etching away the titanium oxide layer 10c with lithography and dry etching techniques.
Further, since the total reflection plate 10 has the glass plate 10a and the titanium oxide layer 10c of which refractive index is higher than the refractive index of the glass plate 10a, the electric field intensity of the evanescent wave is gained at the interface between the titanium oxide layer 10c and the sensing membrane 12.
Consequently, the optical biosensor shown in
Although the invention has been described above by reference to the embodiment of the present invention, the present invention is not limited to the embodiment so described. Modifications and variations of the embodiment so described will occur to those skilled in the art, in the light of the above teachings. Therefore, the scope of the invention is defined with reference to the following claims.
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| Number | Date | Country | |
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| 20060019374 A1 | Jan 2006 | US |
