Determination of thyrotropin in serum by time-resolved fluoroimmunoassay evaluated.

Abstract We evaluated a new, highly sensitive time-resolved fluoroimmunoassay for thyrotropin (TSH) in serum. This direct immunometric "sandwich"-type assay involves two monoclonal antibodies against TSH, one immobilized, the other labeled with europium. Extremely high specific activity of the label and the use of labeled antibody in large excess make the method sensitive enough to measure TSH values falling below the normal reference interval. The standard curve is nearly linear over a wide range of TSH concentrations (standard concentrations range from 0.25 to 324 milli-int. units/L). The lowest concentration detectable was 25 micro-int. units/L. The CV for the assay was less than 6% at 0.5 milli-int. unit/L or higher, 11.3% at 0.1 milli-int. unit/L. For a CV of 10% the lower limit of the working range would be around 0.1 milli-int. unit/L. The interassay CV was 6.7 to 11.8% for TSH concentrations of 0.31 to 19.6 milli-int. units/L. The 95% confidence interval for sera from 111 healthy persons was 0.6-3.8 (range 0.3-3.8) milli-int. units/L. For hyperthyroid patients and thyroid cancer patients treated with thyroxin after thyroidectomy, serum TSH values were all below the reference interval (most were less than 25 micro-int. units/L).

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"Delfia" and "Amerlite": two sensitive nonisotopic immunoassay systems for assay of thyrotropin compared.

Clinical Chemistry ◽

10.1093/clinchem/33.8.1421 ◽

1987 ◽

Vol 33 (8) ◽

pp. 1421-1424 ◽

Cited By ~ 9

Author(s):

A J Parnham ◽

I F Tarbit

Keyword(s):

Quality Assurance ◽

Reference Interval ◽

Regression Equation ◽

Negative Bias ◽

Nonthyroidal Illness ◽

Time Resolved ◽

Standard Curve ◽

Wide Range ◽

Assurance Scheme ◽

Quality Assurance Scheme

Abstract We assessed the LKB "Delfia" (time-resolved dissociation-enhanced lanthanide fluoroimmunoassay) and the Amersham "Amerlite" (enhanced luminescent immunometry) assays of thyrotropin in serum. Both assays are sensitive (respective detection limits: 0.02 and 0.04 milli-int. unit/L) and have very good within- and between-batch precision over a wide range of thyrotropin concentrations. Results by the two methods correlate well (r = 0.992); the regression equation is: Amerlite = 0.915 Delfia - 0.33 milli-int. unit/L. The standard curve for the Delfia assay was linear, but that for the Amerlite assay showed some deviation from linearity below 0.5 milli-int. unit/L. Both assays have a negative bias in comparison with radiolabeled immunoradiometric assays, as judged by results for samples from the Quality Assurance Scheme. Both assays discriminate well between hyper-, hypo-, and euthyroid subjects, and results for thyrotropin for most patients with nonthyroidal illness were within the euthyroid reference interval. Both assays are convenient to perform and are based on systems that provide a viable alternative to radioimmunoassay.

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ULTRAFILTRATION STUDIES OF STEROID-PROTEIN BINDING

Journal of Endocrinology ◽

10.1677/joe.0.0230129 ◽

1961 ◽

Vol 23 (2) ◽

pp. 129-137 ◽

Cited By ~ 56

Author(s):

P. S. CHEN ◽

I. H. MILLS ◽

F. C. BARTTER

Keyword(s):

Protein Binding ◽

Specific Activity ◽

Binding Protein ◽

High Specific Activity ◽

Wide Range

SUMMARY A method is described for determination of the extent of protein binding of steroids by ultrafiltration after addition of radioactively-labelled steroid tracers of high specific activity. Results obtained with specifically labelled 14C-steroids did not differ significantly from those with steroids randomly labelled with tritium. A number of steroids have been studied with this technique. The 'S' shaped curve obtained with some corticosteroids by plotting percentage ultrafilterable against steroid added to the plasma confirmed the presence of the corticosteroid-binding protein which has greater affinity for steroid than albumin. This method of plotting the ultrafiltration data afforded a method of assessing the amount of binding protein (or the number of sites). Cortisone, 17-hydroxy-11-deoxycorticosterone, cortisol, and Δ1 cortisol showed this type of curve. Binding of aldosterone, progesterone and 17-ketosteroids occurred to the same extent in plasma as in 5% albumin. The ultrafilterable fraction of these steroids in plasma was constant over a wide range of total steroid concentration. Binding of testosterone was greater with plasma than with albumin, and did not decrease upon addition of large amounts of testosterone.

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Determination of Fetal Hemoglobin by Time-Resolved Immunofluorometric Assay

Clinical Chemistry ◽

10.1093/clinchem/38.10.2013 ◽

1992 ◽

Vol 38 (10) ◽

pp. 2013-2018 ◽

Cited By ~ 3

Author(s):

U Turpeinen ◽

U H Stenman

Keyword(s):

High Performance ◽

Fetal Hemoglobin ◽

Gamma Chain ◽

Time Resolved ◽

Assay Procedure ◽

Analytical Recovery ◽

Sandwich Type ◽

Capture Antibody ◽

Europium Chelate

Abstract We have developed a "sandwich"-type time-resolved immunofluorometric assay (IFMA) for fetal hemoglobin (HbF) in hemolysates from adults and newborns, amniotic fluid, and plasma, based on a polyclonal and a monoclonal antibody against human fetal hemoglobin. Microtiter wells are coated with polyclonal capture antibody, and the gamma-chain-specific monoclonal tracer antibody is labeled with a europium chelate. In a simple and fast assay procedure, prediluted hemolysates are incubated in the microtiter wells first with capture antibody for 1 h and, after washing, for 1 h with tracer antibody. The wells are washed and the fluorescence of europium is measured. The mean analytical recovery is 102% and results by IFMA agreed well with values obtained by high-performance liquid chromatography. The analytical range of IFMA is large and well suited for clinical purposes. The detection limit of the assay is 0.2 microgram/L and the measuring range extends to 500 micrograms/L.

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The determination of oestradiol and oestrone in the plasma of the domestic fowl by a method involving the use of labelled derivatives

Biochemical Journal ◽

10.1042/bj1060077 ◽

1968 ◽

Vol 106 (1) ◽

pp. 77-86 ◽

Cited By ~ 16

Author(s):

J. E. O'Grady

Keyword(s):

Human Plasma ◽

Paper Chromatography ◽

Domestic Fowl ◽

Specific Activity ◽

High Specific Activity ◽

Double Labelling ◽

Plasma Samples ◽

Labelling Technique ◽

Preliminary Purification

1. A method involving the use of triple-labelled derivatives has been developed for the determination of total oestrone and oestradiol in the plasma of the domestic fowl. The double-labelling technique devised by Svendsen (1960) for the determination of free oestrogens in human plasma was modified to enable the total oestrogen recovery to be determined for each sample. 2. [6,7−3H2]Oestradiol-17β is added to the plasma samples (1–10ml.), which are hydrolysed with acid and the phenolic steroids then extracted and partially purified. The extract is esterified with iodobenzene-p[35S]-sulphonyl chloride of high specific activity. After addition of standard oestrogen [131I]iodobenzene-p-sulphonates the esters are finally purified by paper chromatography. 3. The oestrogens are determined by comparing the 3H/35S and 131I/35S ratios in the purified esters with similar ratios of appropriate standards. 4. With this procedure the recoveries of oestrone and oestradiol after hydrolysis were 70–85% and 72–84% respectively, and after hydrolysis and preliminary purification 38–53% and 39–51% respectively. With this procedure up to 500ng. of oestradiol can be determined. The sensitivity of the technique for oestrone is 3·0ng. and for oestradiol 2·1ng. 5. The ranges of oestradiol and oestrone concentrations found in six plasma samples were 8·3–21·4ng./ml. and 15·2–31·6ng./ml. respectively.

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Measuring thyroxine and thyrotropin simultaneously in a dried blood sample on filter paper, to screen for neonatal hypothyroidism.

Clinical Chemistry ◽

10.1093/clinchem/26.6.0750 ◽

1980 ◽

Vol 26 (6) ◽

pp. 750-753

Author(s):

S Nagataki ◽

K Ishibashi ◽

R Ohsawa ◽

S Suwa ◽

N Tsukamoto ◽

...

Keyword(s):

Filter Paper ◽

Specific Activity ◽

High Specific Activity ◽

High Sensitivity ◽

Recall Rate ◽

Neonatal Hypothyroidism ◽

High Affinity ◽

Follow Up Study ◽

Highly Sensitive

Abstract We have developed a highly sensitive radioimmunoassay of thyroxine and thyrotropin for mass screening for neonatal hypothyroidism. This assay involves a single disc (3 mm diameter) of dried blood on filter paper. The minimum detectable concentrations are 15 pg/tube (10 microgram/L) for thyroxine and 15 nano-int. units/tube (10 milli-int. units/L) for thyrotropin; intra- and interassay CV’s are < 15% in both assays. The high sensitivity of this method is due to use of labeled thyroxine with high specific activity (3 kCi/g) and of an anti-thyrotropin serum with high affinity (Keq = 7.8 × 10(11) L/mol). With this method, 11337 newborns were screened; a follow-up study revealed that only newborns with both high thyrotropin and low thyroxine concentrations had permanent hypothyroidism. We conclude that this method is sensitive, simple, and reliable and that the recall rate with this method is much lower than that of tests for measuring thyroxine or thyrotropin alone.

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Eine Methode zur qualitativen und quantitativen Bestimmung von drei Juvenilhormonen von Insekten

Zeitschrift für Naturforschung C ◽

10.1515/znc-1974-3-412 ◽

1974 ◽

Vol 29 (3-4) ◽

pp. 161-168 ◽

Cited By ~ 41

Author(s):

K. H. Trautmann ◽

A. Schuler ◽

M. Suchý ◽

H.-K. Wipf

Keyword(s):

Quantitative Determination ◽

Specific Activity ◽

High Specific Activity ◽

Ether Extract ◽

Qualitative And Quantitative ◽

Work Up ◽

First Time ◽

Very High ◽

Tenebrio Molitor Larvae

Abstract A method is presented permitting the qualitative and quantitative determination of all three presently known hormones (JH1-3). The determination is based on the method of radioactive isotope dilution, whereby a very small known amount of tritium-labelled JH-1 is added to the ether extract of the particular species. The addition of radioactive JH-1 permits the isolation of all three hormones, because of their similar behaviour during the chosen work up. The quantitative determination was carried out by gas chromatography and the identification was confirmed with the help of retention-times and GC-MS combination. The method was checked by using an extract of Hyalophora cecropia. For the first time methyl 10,11-epoxy-3,7,11-trimethyl-2-trans-6-trans-dodecadienoate (JH-3) could also be identified as the juvenile hormone of Melolontha melolontha. In Vanessa io larvae, Tenebrio molitor larvae and adults and in Musca domestica larvae none of the three known hormones could be detected. The preparation of JH-1 labelled with tritium in the methyl group of the ester was accomplished with very high specific activity (4.34 Ci/mmol) of the tritiated acid with diazomethane.

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A New, Rapid And Sensitive Determination Of Fibrinopeptide- A (FPA) By A High Affinity Antibody To FPA Antiserum

10.1055/s-0038-1652518 ◽

1981 ◽

Author(s):

G Stehle ◽

J Harenberg ◽

H Schmidtgayk ◽

R Zimmermann

Keyword(s):

Rabbit Serum ◽

Normal Rabbit Serum ◽

Standard Curve ◽

High Affinity ◽

Microtiter Plates ◽

Highly Sensitive ◽

Ethanolic Extraction ◽

Sensitive Determination ◽

Radioimmunological Determination

The clinical relevance of the determination of FPA is not yet fully recognized because of the still time consuming radioimmunological techniques. Shortening of the incubation times allways lead to a critical loss of the sensitivity of the assay. We present now a modification which provides highly sensitive and reproducable results within 2hrs.The ethanolic extraction of FPA from plasma was shortened to 20 min including centrifugation. Samples were analysed in triplicates and evaporated at 50°C on microtiter plates. The addition of 0.2μl normal rabbit serum (NRS) lead to a 20% increase of the reaction rate of the FPA antiserum to FPA. A second antibody with high affinity to rabbit immunglobulin i.e. the FPA antiserum improved the maximal binding to 35% after an incubation period of only 10 min. 35-40000 cpm tracer FPA were added to each sample. FPA antiserum, second antibody and NRS were preincubated for 1-24 hrs and then added together with the tracer to the samples. Thus a sensitive standard curve was obtained between 0.16 and 160 ng/ml (12000-600 cpm). The correlation coefficient of this modification to our previously described method was r=0.96 (n=60) The variation coefficient could be improved substantially to 3.1 for low, 4.0 for medium and 4.5% for high FPA. Normal FPA were measured between 0.16 and 2.5 ng/ml (mean 1.4 ng/ml, n=32).The presented modification of the radioimmunological determination of FPA overcomes the difficulties of previously described methods and provides acurate results within 2 hrs.

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Two-site time-resolved immunofluorometric assay of human insulin.

Clinical Chemistry ◽

10.1093/clinchem/32.4.637 ◽

1986 ◽

Vol 32 (4) ◽

pp. 637-640 ◽

Cited By ~ 46

Author(s):

E Toivonen ◽

I Hemmilä ◽

J Marniemi ◽

P N Jørgensen ◽

J Zeuthen ◽

...

Keyword(s):

Human Insulin ◽

Fluorescence Enhancement ◽

Microtiter Plate ◽

The Other ◽

Plasma Samples ◽

Serum Samples ◽

Time Resolved ◽

Standard Curve ◽

Sandwich Type ◽

Plate Strip

Abstract We describe a two-site "sandwich"-type time-resolved immunofluorometric assay for human insulin, based on use of two monoclonal antibodies with different specificities. The first antibody is immobilized on the surface of microtiter plate strip wells, the other is labeled with Eu3+. Serum samples can be assayed with one incubation step; two incubation steps are required when plasma samples are assayed. After the immunoreactions are complete, the bound fraction of Eu3+-label is quantified by dissociating it in a fluorescence-enhancement solution and measuring its fluorescence with a fluorometer with time-resolution. The sensitivity of the assay is 0.24 micro-int. units/mL. The standard curve is linear from 0.24 to 2400 micro-int. units/mL.

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Factor VIII:E113A Represents a High Specific Activity Factor VIII Arising from a Single Point Mutation within a Ca2+ Binding Site.

Blood ◽

10.1182/blood.v104.11.1725.1725 ◽

2004 ◽

Vol 104 (11) ◽

pp. 1725-1725 ◽

Cited By ~ 1

Author(s):

Hironao Wakabayashi ◽

Philip J. Fay

Keyword(s):

Factor Viii ◽

Specific Activity ◽

High Specific Activity ◽

Factor Xa ◽

Saturation Mutagenesis ◽

Single Amino Acid ◽

Single Point Mutation ◽

Wild Type ◽

Activity Increase ◽

Wide Range

Abstract We recently identified an acidic-rich segment in the A1 domain of factor VIII (residues 110-126) that functions in the coordination of Ca2+, an ion necessary for cofactor activity (Wakabayashi et al., J. Biol. Chem.279:12677–12684, 2004). Using Ala-scanning mutagenesis, it was determined that replacement of residue E113 with Ala yielded a factor VIII point mutant that possessed an ~2-fold increased affinity for Ca2+ as compared with wild type, suggesting that this residue did not directly contribute to Ca2+ coordination but rather modulated the affinity of the ion at this site. Furthermore, the E113A factor VIII possessed twice the specific activity of wild type as determined by a one-stage clotting assay. This increased activity was not likely a result of increased affinity for Ca2+, since assays were performed at saturating Ca2+ levels. Saturation mutagenesis at position 113 revealed that substitution at this position with relatively small, nonpolar residues were well-tolerated, whereas replacement with a number of polar or charged residues was detrimental to activity. Ala-substitution yielded the greatest activity increase of ~2-fold and this level was observed over a wide range of factor VIII concentrations. Time course experiments of factor VIII activation following reaction with thrombin revealed similar rates of activation and inactivation of E113A as observed for the wild type. Interestingly, results from factor Xa generation assays using purified reactants showed the mutant possessed <10% greater specific activity than wild type and yielded similar values for Km for substrate factor X, kcat for factor Xa generation and Kd for factor IXa. Thus the single amino acid substitution minimally altered cofactor structure or inter-molecular interactions relating to its participation in factor Xase. These results indicate that mutations within this Ca2+ coordination site may selectively enhance cofactor specific activity as measured in a plasma-based assay compared to activity determined in a purified system. The enhanced activity observed for E113A factor VIII may derive from a subtle alteration in conformation affecting a yet to be identified functional parameter.

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Improvements in the determination of the turnover rate of plasma thyroxine in avian species: application to the Japanese quail

Journal of Endocrinology ◽

10.1677/joe.0.1140191 ◽

1987 ◽

Vol 114 (2) ◽

pp. 191-198 ◽

Cited By ~ 2

Author(s):

E. J. Cookson ◽

J. Glover

Keyword(s):

Japanese Quail ◽

Half Life ◽

Turnover Rate ◽

Specific Activity ◽

Simple Procedure ◽

High Specific Activity ◽

Future Application ◽

Sodium Thiocyanate ◽

Plasma Samples

ABSTRACT The disappearance of the thyroid hormone thyroxine (T4) from plasma in fully grown male Japanese quail can be described as a first order process with a rate constant of 0·178 ± 0·013/h (mean±s.e.m., n = 8), which represents a half-life of 3·90 h. A small amount of [125I]T4 in relation to total circulating T4 was injected i.v. into Japanese quail and plasma samples were taken at appropriate time-intervals for the determination of residual plasma radioactivity. The rate of disappearance of [125I]T4 was subsequently equated to the turnover rate of the endogenous hormone. Previous methods were modified to overcome problems arising from possible disturbance of plasma T4 metabolism, recirculation of radiolabelled iodide, and to purify the [125I]T4 from the plasma samples. By using labelled T4 of very high specific activity, the amount of [125I]T4 administered was kept much smaller than has been used in previous studies on Japanese quail, thus limiting any interference with plasma T4 dynamics. To minimize any disturbance of plasma T4 metabolism, only four blood samples were taken, at three-hourly intervals after the injection of [125I]T4. The rapid turnover of T4 produced a large amount of labelled inorganic iodide, the re-entry of which into the plasma T4 pool was inhibited by s.c. administration of sodium thiocyanate 1 h before injection of[125I]T4. Assay of the true [125I]T4 turnover was significantly improved over that used in previous studies by purifying the [125I]T4 from the plasma samples chromatographically. The samples were applied to small Sephadex G-25 columns with sodium hydroxide (0·1 mol/l) as the eluant. This simple procedure clearly separated the [125I]T4 from the other radioiodinated plasma components such as free iodide, non-hormonal iodinated proteins and triiodothyronine (T3), thus enabling a more accurate assessment of the residual labelled T4 concentration in the plasma and hence the T4 half-life. The future application of this method to the study of plasma T4 turnover under various experimental conditions is discussed and the possible involvement of T4 turnover studies in the assessment of T4 to T3 conversion is considered. J. Endocr. (1987) 114, 191–198

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