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8 results on '"F A Dombrose"'

1. Monoclonal antibodies specific for prothrombin fragment 1.2 and their use in a quantitative enzyme-linked immunosorbent assay

Author

M C Plank, Marcie J. Hursting, J P Steiner, Bryan T. Butman, M L Bell, K M Szewczyk, F A Dombrose, and Bryant M. Moore

Subjects
Immunogen, biology, medicine.diagnostic_test, Chemistry, medicine.drug_class, PROTHROMBIN FRAGMENT 1.2, Biochemistry (medical), Clinical Biochemistry, Monoclonal antibody, Molecular biology, Epitope mapping, Thrombin, Polyclonal antibodies, Immunoassay, biology.protein, medicine, Antibody, medicine.drug
Abstract

Prothrombin fragment 1.2 (F1.2) is an activation peptide generated during a critical event of blood coagulation, the conversion of prothrombin to thrombin. As a marker of thrombin generation, F1.2 has clinical potential in assessing thrombotic risk and monitoring anticoagulant therapy. In developing a highly specific, monoclonal antibody-based immunoassay of human plasma F1.2, we generated six murine anti-F1.2 monoclonal antibodies, using as immunogen a synthetic peptide (sequence: CGSD-RAIEGR) similar to the unique carboxyl terminus of F1.2. Each antibody bound F1.2 but not prothrombin. Epitope mapping studies with one antibody (5-3B) showed that optimum binding required six to eight amino acids plus a terminal arginine to emulate the F1.2 carboxyl terminus. A quantitative sandwich ELISA for human plasma F1.2 was configured with monoclonal antibody 5-3B as the capture antibody and peroxidase-labeled polyclonal antibodies to the F1.2 amino-terminal region as detector antibodies. Calibrators were prepared by adding purified F1.2, 0-10 nmol/L, to F1.2-depleted plasma. Assay characteristics included the following: mean (+/- SD) analytical recovery of 98% +/- 13%; no interference from lipemia, hemolysis, icterus, or thrombolytic agents; 0.08 nmol/L sensitivity; and mean intra- and interassay imprecision (three lots) < 12% at both low and high concentrations of F1.2.

Published
1993

2. Monoclonal antibodies specific for prothrombin fragment 1.2 and their use in a quantitative enzyme-linked immunosorbent assay

Author

M J, Hursting, B T, Butman, J P, Steiner, B M, Moore, M C, Plank, K M, Szewczyk, M L, Bell, and F A, Dombrose

Subjects
Adult, Epitopes, Mice, Mice, Inbred BALB C, Antibody Specificity, Reference Values, Animals, Antibodies, Monoclonal, Humans, Enzyme-Linked Immunosorbent Assay, Prothrombin, Peptide Fragments
Abstract

Prothrombin fragment 1.2 (F1.2) is an activation peptide generated during a critical event of blood coagulation, the conversion of prothrombin to thrombin. As a marker of thrombin generation, F1.2 has clinical potential in assessing thrombotic risk and monitoring anticoagulant therapy. In developing a highly specific, monoclonal antibody-based immunoassay of human plasma F1.2, we generated six murine anti-F1.2 monoclonal antibodies, using as immunogen a synthetic peptide (sequence: CGSD-RAIEGR) similar to the unique carboxyl terminus of F1.2. Each antibody bound F1.2 but not prothrombin. Epitope mapping studies with one antibody (5-3B) showed that optimum binding required six to eight amino acids plus a terminal arginine to emulate the F1.2 carboxyl terminus. A quantitative sandwich ELISA for human plasma F1.2 was configured with monoclonal antibody 5-3B as the capture antibody and peroxidase-labeled polyclonal antibodies to the F1.2 amino-terminal region as detector antibodies. Calibrators were prepared by adding purified F1.2, 0-10 nmol/L, to F1.2-depleted plasma. Assay characteristics included the following: mean (+/- SD) analytical recovery of 98% +/- 13%; no interference from lipemia, hemolysis, icterus, or thrombolytic agents; 0.08 nmol/L sensitivity; and mean intra- and interassay imprecision (three lots)12% at both low and high concentrations of F1.2.

Published
1993

3. The association of bovine prothrombin fragment 1 with phospholipid. Quantitative characterization of the Ca2+ ion-mediated binding of prothrombin fragment 1 to phospholipid vesicles and a molecular model for its association with phospholipids

Author

Sanford N. Gitel, F A Dombrose, K Zawalich, and Craig M. Jackson

Subjects
chemistry.chemical_compound, Phospholipid vesicles, Molecular model, Biochemistry, Chemistry, Phospholipid, Cell Biology, Prothrombin fragment, Molecular Biology
Published
1979

4. A Rapid Screening Method To Increase Efficiency In Assaying Plasma Levels Of Factor VIII Inhibitors

Author

P M Blatt, K S White, and F A Dombrose

Subjects
Chromatography, Chemistry, Screening method, Plasma levels
Abstract

The plasma level of naturally acquired inhibitors to clotting Factor VIII activity (F.VIII: C) was assessed by the Bethesda Inhibitor Assay (BIA). At inhibitor concentrations outside the BIA working range (25% to 75% residual F.VIII: C), patient plasmas had to be diluted. However, when a rough estimate of the inhibitor concentration was unavailable, the choice of dilution was arbitrary and testing became tedious and inefficient. In an effort to improve the BIA, a screening test was devised to predict the appropriate plasma dilution. It is based on the partial thromboplastin time (PTT) of the incubated sample and is performed just prior to preparing dilutions for the F.VIII: C assay. Test plasmas were diluted serially in multiples of two, from 1:2 to 1:1024, and then incubated according to the BIA. After 90 min, samples were removed for PTT determinations to screen for the appropriate dilution to use in the F.VIII: C assay. The first two test dilutions to produce PTT values 21 sec (± 4 sec, 95% confidence interval) greater than the control resulted in a residual F.VIII: C for the BIA within the 25% to 75% acceptable range. When the log ratio of patient-to-control PTT determinations (specific PTT) for a given dilution was plotted as a function of log residual F.VIII: C at that test dilution, in 81 Bethesda assays a linear relationship was observed (p> .25; with r2 = .81). The screening test was 89% effective in predicting an appropriate dilution (range 0 to 1020 Bethesda units/ml). The accuracy can be enhanced further if, based on the first of three dilution screen tests in which the specific PTT >21 sec, the F.VIII: C assay is performed using the middle dilution value first. Depending on whether that dilution yields an acceptable residual F.VIII: C, either the higher or lower dilution is chosen in the second F.VIII: C assay.

Published
1981

6. Antithrombin III And Plasminogen Levels In Moderate And Severe Trauma

Author

A E Seyfer, J Callahan, and F A Dombrose

Subjects
medicine.medical_specialty, Severe trauma, business.industry, Internal medicine, Antithrombin, Medicine, business, Gastroenterology, medicine.drug
Abstract

Functional and immunologic levels of antithrombin III (ATIII) and plasminogen were assessed in three groups of nine patients each: elective surgery, moderate and severe trauma. Patients otherwise healthy were classified as follows: I, elective extremity surgery, no blood transfusions, normal coagulation screening tests (14-50y); II, isolated, moderately severe trauma (e.g., replantation or revascularization of one or more digits), no transfusions (14-56y); and III, Isolated, severe trauma to extremities, with replantation and revascularization of a severed arm or leg, receiving 1-4 units of whole CPD blood (20-59y). Preoperative, intraoperative (2 hr into surgery) and 24 hr postoperative values were measured. Group III only had intraoperative sampling, with the exception of two patients who had preoperative values prior to any transfusions. A detailed statistical comparision was made (at the 95% confidence level) of the differences in ATIII activity, ATIII antigen level, the ratio of ATIII activity-to-antigen and plasminogen activity among categories within and between groups. The data suggest that elective surgery and moderate trauma had virtually the same effect on ATIII and plasminogen. Activity and antigen values decreased intraoperatively but on the average not enough to be out of the acceptable range. During the convalescent period most ATIII values returned to their preoperative level while most plasminogen values continued to decline somewhat (although still in the acceptable range). By contrast, both ATIII and plasminogen values in the severe trauma group were markedly depressed compared to preoperative levels In either group I or II. Four of the patients in this group suffered postoperative thrombosis and loss of an extremity even though the limb was initially viable. The transient lowering of both ATIII and available plasminogen is undoubtedly most critical when surgical stress is superimposed on existing trauma.

Published
1981

7. The association of bovine prothrombin fragment 1 with phospholipid. Quantitative characterization of the Ca2+ ion-mediated binding of prothrombin fragment 1 to phospholipid vesicles and a molecular model for its association with phospholipids

Author

F A, Dombrose, S N, Gitel, K, Zawalich, and C M, Jackson

Subjects
Models, Molecular, Models, Structural, Kinetics, Macromolecular Substances, Animals, Calcium, Cattle, Membranes, Artificial, Prothrombin, Peptide Fragments, Phospholipids, Protein Binding
Published
1979

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