LARNER JOSEPH (US)
BIOCHEMICAL and BIOPHYSICAL RESEARCH COMMUNICATIONS, Volume 151, Number 3, issued 30 March 1988, J. LARNER et al., Dehydrogenase Phosphatase Contains Galactosamine and D-Chiroinositol", pages 1416-1426.
BIOCHEMICAL and BIOPHYSICAL RESEARCH COMMUNCATIONS, Volume 146, Number 2, issued 31 July 1987, J.M. MATO et al., "Partial Structure of an Insulin-Sensitive Glycophospholipid", pages 764-770.
METABOLISM, Volume 35, Number 4, Suppl. 1. issued April 1986. J.R. WILLIAMSON et al., "Diabetes-Induced Increases in Vascular Permeability and Changes in Granulation Tissue Levels of Sorbitol, Mvo-Inositol. Chiro-Inositol, and Scyllo-Inositol are Prevented by Sorbitol" pages 41-45.
Journal of CHROMATOGRAPHY, Volume 277, issued 1983, T. NIWA et al., "Gas Chromatographic-Mass Spectrometric Analysis of Polyols in Urine and Serum of Uremic Patients", pages 25-39.
JOURNAL OF CHROMATOGRAPHY, Volume 336, issued 1984, T. NIWA et al., "Identification of 6-deoxyallitol and 6-deoxygulitol in Human Urine: Electron Impact Mass Spectra of Eight Isomers of 6-deoxyhexitol", pages 345-350.
| 1. | A method for diagnosing mammalian patients for potential insulinresistance associated with a diabetic state, comprising: obtaining a sample from said patient, said sample being selected from the group consisting of a serum sample, and a urine sample, and assaying said sample for the presence of chiro inositol, wherein urinary chiroinositol concentrations below about 1.0 micrograms/ml and serum chiroinositol concentrations below about 0.1 micrograms/ml are indicative of a predisposition to insulinresistance in said patient and serum concentrations of chiroinositol below about 0.1 micrograms/ml. |
| 2. | The process of Claim 1, wherein chiroinositol concentrations in said urine sample at concentrations below about 0.3 micrograms/ml are indicative of insulin¬ resistance in said patient, and wherein chiroinositol concentrations in said urine sample at values between 0.3 micrograms/ml and chiroinositol concentrations in said serum sample below about 0.03 micrograms/ml and about 1 micrograms/ml and serum chiroinositol concentrations between 0.03 0.1 micrograms/ml are indicative of presymptomatic insulinresistance. |
| 3. | The process of Claim 1, wherein said assay step is practiced using an assay selected from the group consisting of gas chromatographic/mass spectrometric analysis, paper chromatography, chiroinositol enzyme specific reduction/oxidation analysis, assays employing antibody specific to chiroinositol, and mixtures thereof. |
| 4. | The process of Claim 3, wherein said assays employing antibody specific to chiroinositol include enzyme linked immunosorbic assays, lypophilic immunosorbent assays and agglutination assays. |
| 5. | A method for screening patients for possible predisposition to the development of insulinresistance, comprising: selecting patients from families having a history of insulinresistance, obtaining a serum or urine sample from said patients, assaying said sample for the presence of chiroinositol, wherein chiroinositol concentrations in said sample below about 1.0 micrograms/ml is indicative of an individual having a predisposition to the development of insulinresistance. |
| 6. | A method for monitoring the efficacy of insulin therapy administered to a diabetic patient, comprising: monitoring the concentration of chiroinositol in said patient over time, wherein a drop in chiroinositol concentration about 1.0 micrograms/ml in the urine of said patient and below about 0.1 micrograms/ml in the serum of said patient is indicative of potential insulin resistance, requiring a suitable treatment alteration. |
Description
Quantitative Analysis of Chiroinositol as a Diabetic Condition Predictor
This is a continuation-in-part of U.S. Patent Application Serial No. 320,485, filed March 8, 1989. The entire disclosure of U.S. Application Serial No. 320,485 is incorporated-by-reference herein.
Technical Field
This invention pertains to a quantitative assay for a marker or predictor of insulin resistance and the associated diabetic condition in mammals, specifically, a quantitative assay which provides for quick screening of individual patients for an indicator of the diabetic state, the absence of chiro-inositol. The assay provides a low-cost, quick method for conducing a preliminary assay for diabetes, or a predilection to the development of diabetes, in mammals, including humans.
Background Art
As reported in parent application Serial No. 320,485, discoveries concerning the structures of insulin mediators in mammals, and the presence, in at least one of those mediators, of D-chiro-inositol, led, in part, to the determination that this particular sugar alcohol was absent, or substantially absent, in diabetic individuals, particularly insulin-resistant diabetics, who traditionally are difflbult to both identify, and treat.
Further research into this phenomenon led to the determination that both D-chiro-inositol and L-chiro- inositol concentrations in diabetic individuals, particularly type II diabetics, are significantly reduced, and that a quantitative assay for the presence
of these "markers" can result in the identification (a) of type II diabetics and (b) individuals at risk or predicted to develop the symptoms of type II diabetes.
U.S. Application Serial No. 320,485, as originally filed, discloses one type of sample to be screened for the presence of D-chiro-inositol. This includes the collection of a 24-hour urine sample, accompanied by convenience of frozen storage, if necessary. Although highly desirable, due to its non-invasive nature, low cost, reliability and speed, further improvements on this process could be obtained.
Accordingly, it remains an object of those of ordinary skill in the art to provide a sensitive, quantitative assay for both D and L-chiro-inositol, as a marker, indicator or predictor of insulin-resistance and type II diabetes.
Disclosure of the Invention
The above objects, and others more fully developed below, are achieved by a quantitative assay for chiro- inositol taken from spot samples of either mammalian urine or serum. Concentrations of chiro-inositol, relative to both normal individuals, and other inositols, appear constant in both types of samples, eliminating the need for a 24-hour urine specimen collection, and providing alternative fluid sources, both for the convenience of the analyst, and for a check on assay results.
One convenient assay system involves the use of conventional gas chromatography/mass spectrophotometry (GC/MS) . Other assay methods are known. Chiro-inositol
1/12 35
-3-
concentrations of 1 micrograms/ml and above in either urine or serum samples is indicative of the normal or control concentrations for chiro-inositols in healthy individuals. A value of 0.3 icrograms - 1 micrograms per ml is suggestive of a mammalian individual at risk for the development of type II diabetes, or may be further indicative of a presymptomatic type II diabetic. Chiro-inositol values below 0.3 micrograms/ml are indicative of type II diabetics. Chiro-inositol concentrations in serum samples are about 10 fold lower than urine. Thus, values in serum of below 0.1 micrograms/ml are indicative of individuals at risk, and values below about 0.03 are- indicative of type II diabetes.
It has further been discovered that similar low inositol concentrations can be correlated with type I diabetics demonstrating insulin-resistance, a characteristic of type II diabetics. Thus, sampling of mammalian populations according to the quantitative assay of this invention appears to be indicative of insulin-resistance, exhibited by a 1- ited number of type I diabetics and type II diabetics. Accordingly, the assay may be used both as a confirmatory assay for the presence of type II diabetes in all populations, a confirmation for insulin-resistance in type I diabetics not responding to insulin therapy, as well as a useful tool for family studies and genetic prediction for insulin-resistant individuals, or individuals drawn from families exhibiting insulin-resistance, for generational planning.
Best Mode for Carrvinσ Out The Invention
In the performance of the assay of this invention, a urine or serum sample must be obtained. These samples may be spot samples, and no specific time of day or fasting period is required in order to perform the assay with accuracy and precision. Additionally, concentrations of chiro-inositol in patients exhibiting below normal concentrations appear to be independent of various sugar-lowering agents, including insulin and related agents. If a urine sample is obtained, the sample may be adsorbed onto a conventional anion/cation exchange resin bed, eluted with distilled deionized water, and further purified, through solid phase extraction. The sample collection is recovered in distilled water, dried and derivatized. An exemplary derivatization material is heptafluorobutyrlimidazole. In an alternative embodiment of the invention, a serum sample may be collected and subjected, e.g., to ultrafiltration and then applied to purification resins, and subsequently derivatized, as with the urine specimen discussed above.
Conventionally, the samples prepared may be easily assayed on a gas chromatography/mass spectrometer (e.g. HP5710A chromatograph combined with a JMS D-300JEOL spectrometer) .
Spot samples exhibiting chiro-inositol concentration (D- and L- combined) of about 1 micrograms/ml and above are representative of normal concentrations, exhibited by non-diabetic, non-insulin- resistant individuals. Assays reflecting values below about 0.3 micrograms/ml are insulin-resistant. Type I diabetics exhibiting these substantially absent chiro- inositol concentrations should be considered insulin- resistant, when determining proper therapy. The
remaining individuals are expected to be type II diabetics.
Values obtained through the assay of this invention of 0.3 micrograms - 1 micrograms/ml are indicative of individuals at risk of development of type II diabetes, or individuals who are presymptomatic type II diabetics. All such readings should be confirmed, of course, by subsequent more involved assays available to those of skill in the art.
Studies on Pima indian populations of Arizona, as well as a patient population in and about the University of Virginia, Charlottesville, Virginia, and diabetic rhesus monkeys, University of Maryland Primate Center, exhibit a virtual absence of chiro-inositol in diabetic individuals. The marked correlation between chiro- inositol concentrations and insulin-resistance, through these blindrblind studies, was particularly dramatic when compared with the concentrations of structurally related myo-inositol concentrations, which are generally elevated in diabetic patients, and were significantly higher in the diabetic subjects studied than non- diabetics.
Muscle biopsy experiments confirm the findings of low or nonexistent concentrations of chiro-inositol in the patients studied exhibiting non-insulin dependent diabetes mellitus (NIDDM) . Given the apparent presence of chiro-inositol in insulin mediators and the correlation between the absence of chiro-inositol and insulin-resistance, applicants believe that there may be a biosynthesis pathway lacking in individuals exhibiting NIDDM and related insulin-resistance or insulin insensitivity, which prevents or retards the formation
*
• . -6-
of a mediator essential in some insulin-activated metabolic pathways. Applicants do not wish to be bound by this theory.
The importance of chiro-inositol as a compound linked to insulin-resistance, and thus linked to individuals requiring non-insulin therapy in the treatment of diabetes, provides a convenient method of monitoring the efficacy of chemical therapy prescribed for the diabetic patient. Those diabetics under some type of chemical therapy, including insulin administration, can be monitored routinely through the assay of this invention for chiro-inositol concentrations. A pronounced drop in the chiro-inositol concentrations, or absence of chiro-inositol from the serum, urine or other sample, is suggestive of insulin- resistance. Additionally, if the individual is on an inositol supplement, in order to treat the deficiency, assays of samples taken some hours subsequent to ingestion of the medication should give an accurate reflection of the value of the treatment.
It should be noted that this invention can be practiced through assays other than GC/MS. A wide variety of assays are known to those of ordinary skill in the art for the detection of specific compounds, and the use of any one which is consistent with a derivatized, dried or liquid sample is appropriate herein. Thus, enzyme reduction/oxidation potential measurements, using, e.g., an immobilized enzyme specific for chiro-inositol, the immobilized enzyme being in a fixed relationship to an electrode, may be used. The presence of chiro-inositol will result in the enzyme-catalyzed reaction going forward, altering the electrical environment detected by the electrode.
Alternative assays that can be employed may include antibody assays, e.g., ELISA, LISA, agglutination assays and the like. All such assays are within the context of the invention claimed herein.
The above invention has been described with reference to specific examples and materials. It should be clear that these specifics can be varied without departing from the scope of the invention. In particular, alternative resins in the purification format, alternation of the -purification sequence, and alternative assay forms, sensitive to chiro-inositol may be employed, without departing from the scope of the invention, as defined by the claims appended hereto.
Next Patent: IMMUNOCHROMATOGRAPHIC ASSAY AND METHOD OF USING SAME