Maj-Gret I. Welin’s research while affiliated with Covidien Finland Oy and other places

What is this page?


This page lists works of an author who doesn't have a ResearchGate profile or hasn't added the works to their profile yet. It is automatically generated from public (personal) data to further our legitimate goal of comprehensive and accurate scientific recordkeeping. If you are this author and want this page removed, please let us know.

Publications (4)


A rapid fluorometric enzyme immunoassay for the determination of neonatal TSH from blood spots
  • Article

November 1991

·

37 Reads

·

7 Citations

Clinica Chimica Acta

·

·

Maj-Gret I. Welin

·

[...]

·

Kirsti I. Käpyaho

We describe a novel method for the detection of thyrotropin from dried blood spots using a horseradish peroxidase-labelled sandwich enzyme immunoassay with fluorometric detection. The detection limit of the present assay is 1.25 mIU/l with within-run and between-run imprecision being in the range 5.2 to 11.4%. The results of the assay correlate well with two commercial methods: an enzyme immunoassay (r = 0.93) and a time-resolved fluorescence assay (r = 0.90). The blood spot values also show a good correlation (r = 0.93) with respective values obtained from plasma using a commercial immunoradiometric method.The assay may also be performed colorimetrically with sensitivity similar to the fluorometric assay. However, the latter provides a wider dynamic range with an upper limit of 400 mIU/l while the colorimetric method reaches a plateau at 25 mIU/l. Due to its simplicity and rapid performance (3 h), the fluorometric assay is suitable for the routine screening of congenital hypothyroidism.


3-p-Hydroxyphenylpropionic Acid—A Sensitive Fluorogenic Substrate for Automated Fluorometric Enzyme Immunoassays

February 1991

·

61 Reads

·

19 Citations

Journal of Immunoassay

The application of 3-p-hydroxyphenylpropionic acid (HPPA), a fluorogenic substrate of horseradish peroxidase (HRP) to an automated microplate fluorometric enzyme immunoassay is described. Fluorescence intensity of the end product was highly dependent on the pH of the buffer and on the concentrations of the substrate mixture ingredients. The determination of human thyrotropin (TSH) and recombinant hepatitis B surface antigen (rHBsAg) were performed using a fluorometric enzyme immunoassay (FEIA) with HPPA as the substrate, and a colorimetric one with tetramethylbenzidine (TMB) as the chromogenic substrate. The sensitivity of both types of assays proved comparable. The distinct advantage of a fluorometric assay is the possibility to perform a quantitative detection of analyte over a very wide dynamic range. Clinical evaluation of both assays showed good correlation between the FEIA and conventional methods.


Rapid determination of C-reactive protein by enzyme immunoassay using two monoclonal antibodies

July 1989

·

16 Reads

·

21 Citations

Scandinavian Journal of Clinical and Laboratory Investigation

Several monoclonal antibodies for human C-reactive protein (CRP) were characterized, and two antibodies binding to separate domains were used to construct a rapid and simple immunoenzymometric assay for CRP. The assay consists of a single 15 min immunological reaction during which CRP forms a complex with a peroxidase-labelled antibody and with another antibody attached to the test-tube wall. The immobilized complex is detected by a 3 min colour reaction using peroxidase substrate. The quantitative measuring range of the assay is 0.04-5 mg/l, and no hook occurs at five-fold higher values. The sensitivity of the method allows reliable determination of low CRP levels, eg. in paediatric samples. The values obtained with the present assay correlated well with turbidimetric results.


Monoclonal antibodies to the 27–34K insulin-like growth factor binding protein

May 1988

·

12 Reads

·

56 Citations

Biochemical and Biophysical Research Communications

Monoclonal antibodies were prepared against the 27-34K insulin-like growth factor (IGF)-binding protein purified from human placenta/decidua and designated placental protein 12 (PP12). Four different antibodies were characterized. Each recognized the major band at 32K on immunoblots of the purified PP12 preparation and amniotic fluid. In liquid phase RIA, IGF-I did not affect the binding of [125I] PP12 to one antibody (Mab 6303), it slightly increased the binding to two antibodies (Mab 6301 and 6304), and it slightly decreased the binding to one antibody (Mab 6302). All antibodies immunoprecipitated the cross-linked PP12-[125I] IGF-I complex, but Mab 6302 considerably less effectively than the others. Preincubation of PP12 with Mab 6302 completely inhibited the binding of [125I] IGF-I to PP12, whereas preincubation with Mab 6303 had no effect, and Mab 6301 as well as Mab 6304 increased it. These results suggest that Mab 6302 binds to an epitope at or near to the IGF-binding site, whereas the other antibodies react at other sites of the PP12 molecule. Conformational changes in PP12 probably account for the IGF-I-induced increase in the binding of Mabs 6301 and 6304 to [125I] PP12, and vice versa, for Mabs 6301- and 6304-induced increase in the binding of [125I] IGF-I to PP12.

Citations (4)


... Using of DBS technology for the preparation and analysis of target antigens in dried blood spots by immunoassay for the purposes of medical and veterinary diagnostics was described earlier. [16][17][18][19][20][21] DBS cards of conventional format are manufactured with cellulose bres and samples are applied dropwise onto marked round parts of the card. Aer drying, the paper discs with applied sample are punched. ...

Reference:

Porous membrane strip microsampling: A dried biofluid collection format and application for quantitative enzyme immunoassay
A rapid fluorometric enzyme immunoassay for the determination of neonatal TSH from blood spots
  • Citing Article
  • November 1991

Clinica Chimica Acta

... The adaptation to HRP was attempted by Zapata and co-workers using 4-hydroxybenzoic acid (HBA) [5]. The oxidation products of 4-hydroxyphenylpropionic acid (pHPPA) [6], chavicol [7], Amplex red [8] and prochlorperazine [9] did not sensitize their fluorescence measurements in the corresponding experiment setup. The other common drawbacks of aforementioned fluorogenic substrates are their insufficient reaction rates, relatively low stability in air or toward H 2 O 2 in the absence of HRP, tending to cause strong background signals and poor water-solubility [10,11]. ...

3-p-Hydroxyphenylpropionic Acid—A Sensitive Fluorogenic Substrate for Automated Fluorometric Enzyme Immunoassays
  • Citing Article
  • February 1991

Journal of Immunoassay

... IGFBP-1, which is a major protein of human decidua, constitutes a subgroup of the IGFBP system. IGFBP-1 has a higher concentration in amniotic fluid than in serum; its concentration gradually increases in the amniotic fluid in the mid-trimester in comparison with its concentration in the maternal plasma 24 . ...

Monoclonal antibodies to the 27–34K insulin-like growth factor binding protein
  • Citing Article
  • May 1988

Biochemical and Biophysical Research Communications

... The selected anti-CRP mAb has an ultrahigh picomolar level affinity for CRP binding. 29 Similar to the bio-BSA/SA pair, the binding between CRP and the specific anti-CRP mAb resulted in an increase in the TRL-signal at RT, whereas the nonspecific mAbs had no significant impact on the signal (Figure 3, Figure S2). Within the studied concentration ranges, the observed TRL signal between the protein complex and mAb alone peaked at the approximate ratio of 5:1 (mAb/CRP) independent of the protein concentration level. ...

Rapid determination of C-reactive protein by enzyme immunoassay using two monoclonal antibodies
  • Citing Article
  • July 1989

Scandinavian Journal of Clinical and Laboratory Investigation