Your search keyword '"M J Khosravi"' showing total 10 results

1. Noncompetitive ELISA for human serum insulin-like growth factor-I

Author

J. Mistry, Anastasia Diamandi, Phillip Lee, and M. J. Khosravi

Subjects

Chromatography, biology, medicine.diagnostic_test, Growth factor, medicine.medical_treatment, Biochemistry (medical), Clinical Biochemistry, Extraction (chemistry), Insulin-like growth factor-binding protein, Immunoassay, biology.protein, medicine, Centrifugation, Sample preparation, Antibody, Quantitative analysis (chemistry)

Abstract

Measurement of serum insulin-like growth factor I (IGF-I) is important in assessing the growth hormone/IGF axis. Competitive immunoassay methods for IGF-I are complicated by substantial interference from IGF-binding proteins (IGFBPs) due to the relatively low ratio of specific antibody to IGFBPs in the sample, even after standard acid-ethanol sample extraction. We report of development of a noncompetitive ELISA for human IGF-I that avoids this problem by utilizing excess amounts of capture and detection antibodies. Serum samples were prepared by using an abbreviated acid-ethanol extraction method. Neutralized supernatant was added to microwells coated with IGF-I capture antibody; horseradish peroxidase-labeled detection antibody was then added, incubated for 2 h, and then developed. Compared with the "gold standard" method of acid-column chromatography, the simplified acid-ethanol extraction yields a mean +/- SD recovery of 103% +/- 5.5% despite the presence of residual IGFBPs in the extracted sample. Comparisons with a centrifugal filtration sample extraction method are also shown. The ELISA is specific for IGF-I with an absolute sensitivity of 0.03 microgram/L and inter- and intraassay CVs of 3.9-8.8% and 2.6-6.7%, respectively. The availability of a rapid IGF-I ELISA combined with a simple and reliable sample preparation procedure should facilitate clinical and research studies of this important growth factor.

Published

1996

2. Associations between insulin-like growth factors and their binding proteins and other prognostic indicators in breast cancer

Author

Eleftherios P. Diamandis, Gary M. Clark, He Yu, Michael A. Levesque, A. Papanastasiou-Diamandi, and M J Khosravi

Subjects

Cancer Research, medicine.medical_specialty, Receptor, ErbB-2, medicine.medical_treatment, Mammary gland, Breast Neoplasms, Biology, Cathepsin D, Insulin-like growth factor-binding protein, S Phase, Breast cancer, Somatomedins, Internal medicine, medicine, Biomarkers, Tumor, Humans, Epidermal growth factor receptor, Receptor, Ploidies, Growth factor, DNA, Neoplasm, medicine.disease, Prognosis, ErbB Receptors, Insulin-Like Growth Factor Binding Proteins, Steroid hormone, medicine.anatomical_structure, Endocrinology, Oncology, Receptors, Estrogen, Insulin-like growth factor 2, Cancer research, biology.protein, Female, Tumor Suppressor Protein p53, Receptors, Progesterone, hormones, hormone substitutes, and hormone antagonists, Research Article

Abstract

Recent studies have suggested that insulin-like growth factors (IGFs) and insulin-like growth factor binding proteins (IGFBPs) may be implicated in the development and progression of breast cancer. Prostate-specific antigen (PSA), a serine protease, may play a role in the regulation of IGFs' function through cleavage of IGFBP-3, resulting in release of active IGFs from IGFBP-3. As IGFs, IGFBPs and PSA are all present in breast cancer, possible associations among these proteins were speculated. In this study, we have measured PSA, IGF-I, IGF-II, IGFBP-1 and IGFBP-3 in tumour tissue cytosols from 200 women with primary breast cancer, and have examined relationships between IGFs or IGFBPs and PSA along with other markers, including p53 protein, steroid hormone receptors (oestrogen and progesterone), cathepsin-D, epidermal growth factor receptor, Her-2/neu protein, S-phase fraction and DNA ploidy. Correlations or associations between PSA and IGF-I, IGF-II, IGFBP-1 or IGFBP-3 were not observed. IGF-II was positively correlated with both IGFBP-3 and IGFBP-1. IGF-I was not associated with either of the two binding proteins, nor with IGF-II. Both IGF-II and IGFBP-3 were inversely associated with the oestrogen receptor, and IGFBP-3 was also positively associated with S-phase fraction. Our finding of IGF-II and IGFBP-3 in association with unfavourable prognostic indicators of breast cancer suggests that IGFs may be involved in the progression of breast cancer.

Published

1996

3. Hapten-heterologous conjugates evaluated for application to free thyroxine immunoassays

Author

A Papanastasiou-Diamandi and M J Khosravi

Subjects

biology, medicine.drug_class, Chemistry, Biochemistry (medical), Clinical Biochemistry, Heterologous, Radioimmunoassay, Monoclonal antibody, Antigen, Biochemistry, Biotinylation, medicine, biology.protein, Antibody, Hapten, Conjugate

Abstract

We evaluated the effect of hapten heterology on free thyroxine (FT4) immunoassays involving the biotin-streptavidin system and time-resolved fluorometry. We compared protein derivatives of thyroxine (T4) and triiodothyronine (T3) as solid-phase antigen or biotinylated protein-tracer conjugate for competitive (or sequential) binding to a mouse anti-T4 monoclonal antibody. In both one- and two-step assays, the heterologous combination of the antibody and T3 conjugates showed superior standard curve sensitivity but up to eightfold lower zero standard signal (B(o)) when the same amounts of antibody and conjugates were used. The improved sensitivity was not altered when the amount of coupled T3 was increased to obtain a B(o) value similar to that of the homologous combination of antibody and T4 conjugates. In the two-step format, the sensitivity of the homologous assay was insufficient for routine use, consistent with displacement of bound T4 during the antibody back-titration step (demonstrated in the T4 displacement experiment with excess conjugate). Results from the one-step (labeled antibody) heterologous assay for approximately 85 clinical samples correlated well with those from an immunofluorometric assay and a two-step radioimmunoassay. The assay was not affected by a wide variation in endogenous serum concentrations of T4-binding globulin and albumin.

Published

1993

4. Novel application of streptavidin-hapten derivatives as protein-tracer conjugate in competitive-type immunoassays involving biotinylated detection probes

Author

M J Khosravi and R C Morton

Subjects

Streptavidin, Chromatography, biology, Biochemistry (medical), Clinical Biochemistry, Fluorescence spectroscopy, chemistry.chemical_compound, Biotin, chemistry, Biotinylation, Reagent, biology.protein, Hapten, Avidin, Conjugate

Abstract

To investigate the use of streptavidin-hapten derivatives as potential protein-tracer conjugates for competitive-type immunoassays, we labeled streptavidin with cortisol and compared biotin-binding activity of the conjugates with that of unlabeled streptavidin. In this model system, streptavidin labeled with one to approximately 17 cortisol molecules retained its capability to cross-link a biotinylated protein on microtiter wells to a biotin-based general detection reagent developed for time-resolved fluorometry. Compared with unlabeled streptavidin, there was no reduction in the binding activity of the conjugate carrying as many as 2.6 cortisol molecules per molecule of streptavidin. Conjugation ratios greater than 4.4 showed a slight decrease in binding activity, presumably because of the aggregate formation evident at these labeling ratios. As expected, the conjugates were also capable of linking a solid-phase-bound anti-cortisol monoclonal antibody to the biotinylated detection reagent. The fluorescence signal generated increased almost linearly with increasing conjugation ratios from about three to nine cortisol molecules per molecule of streptavidin. At greater ratios, the assay response plateaued. The calibration curves obtained were typical for competitive-type immunoassays when the conjugates were incorporated in a cortisol assay based on a second-antibody immobilization approach.

Published

1991

5. Acid-labile subunit of human insulin-like growth factor-binding protein complex: measurement, molecular, and clinical evaluation

Author

Anastasia Diamandi, Radha G. Krishna, M. J. Khosravi, A Khare, and Jehangir Mistry

Subjects

Adult, Male, Endocrinology, Diabetes and Metabolism, Protein subunit, Clinical Biochemistry, Size-exclusion chromatography, Molecular Conformation, Enzyme-Linked Immunosorbent Assay, Biochemistry, High-performance liquid chromatography, Insulin-like growth factor-binding protein, Endocrinology, Affinity chromatography, Insulin-Like Growth Factor II, Synovial fluid, Humans, Insulin-Like Growth Factor I, Aged, Glycoproteins, biology, Chemistry, Human Growth Hormone, Binding protein, Biochemistry (medical), Middle Aged, Molecular biology, Insulin-Like Growth Factor Binding Protein 3, Acromegaly, biology.protein, Female, Carrier Proteins, Quantitative analysis (chemistry)

Abstract

Although the acid-labile subunit (ALS) of the approximately 150-kDa insulin-like growth factor (IGF)-binding protein (IGFBP) complex was described over a decade ago, details of ALS physiology have remained largely uncertain. We evaluated antibodies to synthetic human ALS and constructed a noncompetitive ALS enzyme-linked immunosorbent assay. Whereas uncomplexed ALS is directly measured, determination of total levels required sample pretreatment with SDS, which was found to optimally dissociate complexed ALS and significantly enhance ALS immunoreactivity. ALS in random adult sera was approximately 50% uncomplexed, and samples devoid of complexed ALS by immunoaffinity separation contained about 54% of the total levels. Serum ALS fractionated by gel filtration high performance liquid chromatography eluted in a single peak at approximately 150 kDa with IGF-I and IGFBP-3, but appeared at about 400-500 kDa after sample acidification and fractionation under acidic condition. The unexpected shift in ALS immunoreactivity remained unchanged when acid-neutralized or SDS-treated samples were fractionated under neutral pH and was reproducible when the 150-kDa complex was isolated, treated with acid or SDS, and rechromatographed. ALS in adult sera more tightly correlated with IGFBP-3 than IGF-I or IGF-II. The total levels (mean +/- SD) were 16.7 +/- 3.7 mg/L in 22 normal subjects, 28.3 +/- 8.1 mg/L in 20 acromegalic patients, and 9.5 +/- 3.8 in 32 GH-deficient adults. Little or no ALS was detectable in amniotic fluid, cerebrospinal fluid, seminal plasma, or milk, whereas high levels were present in synovial fluid. The development of ALS enzyme-linked immunosorbent assay should greatly facilitate further investigations of this unique glycoprotein.

Published

1997

6. An ultrasensitive immunoassay for prostate-specific antigen based on conventional colorimetric detection

Author

M J Khosravi, J Mistry, and A Papanastasiou-Diamandi

Subjects

Male, medicine.drug_class, Clinical Biochemistry, Chemical Fractionation, Monoclonal antibody, Horseradish peroxidase, Antibodies, medicine, Humans, Colorimetry, Peroxidase, Detection limit, Immunoassay, Prostatectomy, biology, medicine.diagnostic_test, Chemistry, Antibodies, Monoclonal, General Medicine, Prostate-Specific Antigen, Molecular biology, Prostate-specific antigen, Polyclonal antibodies, biology.protein, Female, Antibody

Abstract

Development of an ultrasensitive immunoassay for serum PSA involving conventional detection probes.The assay involves a polyclonal antibody immobilized in microtitration wells and a monoclonal antibody labeled with horseradish peroxidase. In a one-step assay, the enzymatic activity of the bound detection antibody is monitored by the addition of hydrogen peroxide/tetramethylbenzidine substrate reagent followed by spectrophotometric quantification of the conversion product.The assay has a lower detection limit of 0.003 micrograms/L, biological detection limit of 0.009 micrograms/L, and intra- and interassay CVs of 8.2% and 10.5% at PSA concentrations of 0.022 and 0.065 micrograms/L, respectively. The recovery of the assay averaged 104% and it demonstrated a dilution linearity down to at least 0.01 micrograms of PSA/L. Results of comparison data correlated well with those obtained by a well established enzyme immunoassay. The serum PSA concentrations were0.012 micrograms/L in the majority of patients (53.8%) who had undergone radical prostatectomy.This assay is well suited for post-surgical monitoring of PSA in patients with prostate cancer.

Published

1995

7. Detection of immunoglobulins G and M to rubella virus by time-resolved immunofluorometry

Author

M J Khosravi, Esther Reichstein, P Shankaran, and Eleftherios P. Diamandis

Subjects

Microbiology (medical), Streptavidin, medicine.drug_class, Dose-Response Relationship, Immunologic, Fluorescent Antibody Technique, Enzyme-Linked Immunosorbent Assay, Biology, Monoclonal antibody, medicine.disease_cause, Immunofluorescence, Antibodies, Viral, Rubella, Immunoglobulin G, chemistry.chemical_compound, Predictive Value of Tests, medicine, Humans, Antigens, Viral, medicine.diagnostic_test, Rubella virus, medicine.disease, Virology, Molecular biology, chemistry, Immunoglobulin M, Biotinylation, biology.protein, Reagent Kits, Diagnostic, Antibody, Latex Fixation Tests, Research Article

Abstract

We describe new methods for the detection of immunoglobulin G (IgG) and IgM rubella-specific antibodies in serum. The IgG assay was based on a solid-phase rubella antigen immobilization approach, and the IgM assay was based on the IgM capture assay principle. Both assays used biotinylated antibodies (anti-human IgG and antirubella monoclonal antibody, respectively). The tracer system was based on streptavidin labeled with a fluorescent europium chelate. The final measurements were done by using time-resolved fluorescence. Both assays were thoroughly evaluated with clinical samples and compared successfully with established techniques. We anticipate that these assays are suitable for routine clinical use.

Published

1990

8. A sensitive time-resolved immunofluorometric assay of ferritin in serum with monoclonal antibodies

Author

Marcia A. Chan, M J Khosravi, Eleftherios P. Diamandis, and Astrid C. Bellem

Subjects

Streptavidin, medicine.drug_class, Clinical Biochemistry, Radioimmunoassay, Buffers, Cross Reactions, Monoclonal antibody, Biochemistry, chemistry.chemical_compound, Fluorometer, medicine, Humans, Fluorometry, Immunoassay, biology, medicine.diagnostic_test, Biochemistry (medical), Antibodies, Monoclonal, General Medicine, Molecular biology, Ferritin, chemistry, Biotinylation, Ferritins, Monoclonal, biology.protein

Abstract

We describe a new non-isotopic immunoassay for the quantitation of ferritin in serum. Ferritin is first immunoextracted from serum with a monoclonal antibody immobilized in white microtiter wells. A second biotinylated antibody is then added. The bound biotinylated antibody is quantified by a bridge reaction with streptavidin labeled with the europium chelate 4,7-bis(chlorosulfophenyl)-1,10-phenanthroline-2,9-dicarboxylic acid (BCPDA) in the presence of excess Eu3+. The fluorescence on the bottom of the dry microtiter well consisting of monoclonal antibody-ferritin-monoclonal antibody-biotin-streptavidin-BCPDA-Eu3+ is then measured with a time-resolved fluorometer. The assay is sensitive (0.5 microgram/l), precise (CV's 3-9%) and accurate (average recovery 102%). Results compared well (r = 0.99) with those of a widely used RIA procedure.

Published

1988

9. Time-Resolved Immunofluorometric Assay for Thyroxine-Binding Globulin in Serum

Author

Yok K. Tan, M J Khosravi, and Eleftherios P. Diamandis

Subjects

Pharmacology, Detection limit, Streptavidin, Chromatography, Globulin, biology, Chemistry, Fluoroimmunoassay, Immunology, Fluorescence spectrometry, Radioimmunoassay, Thyroxine-Binding Proteins, chemistry.chemical_compound, Thyroxine-binding globulin, Evaluation Studies as Topic, Fluorometer, Biotinylation, biology.protein, Humans

Abstract

We describe a new "sandwich"-type immunofluorometric assay for thyroxine-binding globulin (TBG) in serum. The assay involves a solid-phase monoclonal antibody immobilised in white microtiter wells, and a soluble biotinylated monoclonal antibody that reacts with the captured TBG molecules. Addition of streptavidin labeled with the europium chelator, BCPDA (4,7-bis(chlorosulfophenyl)-1,10 phenanthroline-2,9-dicarboxylic acid), and excess europium results in the formation of a highly fluorescent product. The fluorescence signal of the final complex is quantitated on the dried solid-phase with a pulsed-laser time-resolved fluorometer. The assay requires a 151-fold sample pre-dilution and a total incubation time of 90 minutes. It has a broad dynamic range of 0-100 mg/L and a minimum detection limit of 0.4 mg/L. The coefficients of variation for within-run and between-run assays averaged 4.5% and 5.4%, respectively. The mean analytical recovery of TBG added to serum was 103%. Results obtained by this method correlated well with those determined by a commercial radioimmunoassay (r = 0.96, n = 112) and by an immunoradiometric procedure (r = 0.95, n = 131).

Published

1989

10. Time-resolved immunofluorometric assay of human pancreatic isoamylase in serum, with use of two monoclonal antibodies

Author

M J Khosravi, A. Papanastasiou-Diamandi, V Lustig, A Tan, and Eleftherios P. Diamandis

Subjects

Streptavidin, biology, medicine.diagnostic_test, medicine.drug_class, Biochemistry (medical), Clinical Biochemistry, Immunofluorescence, Monoclonal antibody, Enzyme assay, chemistry.chemical_compound, Biochemistry, chemistry, Biotinylation, biology.protein, medicine, Isoamylase, Amylase, Antibody

Abstract

This new method for determining pancreatic isoamylase (EC 3.2.1.1) in serum involves two monoclonal antibodies: one immobilized in a microtitration well (the capture antibody), the other biotinylated. After the sample is incubated with the two antibodies, the captured immunocomplex is quantified by adding streptavidin labeled with a europium chelator and measuring the specific Eu3+ fluorescence in a time-resolved mode. Three assay protocols are proposed, involving incubation times of 90, 45, or 25 min. The assay has low (0.005%) cross-reactivity with the salivary isoenzyme. Analytical performance was satisfactory. Results correlate well with results obtained by measuring total amylase activity or by measuring pancreatic isoamylase activity after immunoinhibition. Unlike numerous current amylase assays, this method measures enzyme mass rather than enzyme activity. Potentially, this is a highly specific assay.

Published

1989