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4 research outputs found

Production and Characterization of Peptide Antibodies to the C-Terminal of Frameshifted Calreticulin Associated with Myeloproliferative Diseases

Author: Bergmann Ann Christina
Ciplys Evaldas
Friis Tina
Hansen Paul Robert
Holmström Morten Orebo
Houen Gunnar
Huynh Ha Uyen Buu
Højrup Peter
Jørgensen Sarah Hyllekvist
Kesmez Meliha
Mansha Inaam
Mughal Farah Perveen
Schürch Patrick Mark
Slibinskas Rimantas
Theocharides Alexandre Pierre André
Trier Nicole Hartwig
Publication venue: 'MDPI AG'
Publication date: 18/06/2022
Field of study

Myeloproliferative Neoplasms (MPNs) constitute a group of rare blood cancers that are characterized by mutations in bone marrow stem cells leading to the overproduction of erythrocytes, leukocytes, and thrombocytes. Mutations in calreticulin (CRT) genes may initiate MPNs, causing a novel variable polybasic stretch terminating in a common C-terminal sequence in the frameshifted CRT (CRTfs) proteins. Peptide antibodies to the mutated C-terminal are important reagents for research in the molecular mechanisms of MPNs and for the development of new diagnostic assays and therapies. In this study, eight peptide antibodies targeting the C-terminal of CRTfs were produced and characterised by modified enzyme-linked immunosorbent assays using resin-bound peptides. The antibodies reacted to two epitopes: CREACLQGWTE for SSI-HYB 385-01, 385-02, 385-03, 385-04, 385-07, 385-08, and 385-09 and CLQGWT for SSI-HYB 385-06. For the majority of antibodies, the residues Cys1, Trp9, and Glu11 were essential for reactivity. SSI-HYB 385-06, with the highest affinity, recognised recombinant CRTfs produced in yeast and the MARIMO cell line expressing CRTfs when examined in Western immunoblotting. Moreover, SSI-HYB 385-06 occasionally reacted to CRTfs from MPN patients when analysed by flow cytometry. The characterized antibodies may be used to understand the role of CRTfs in the pathogenesis of MPNs and to design and develop new diagnostic assays and therapeutic targets. Keywords: calreticulin; epitope mapping; frameshift mutations; myeloproliferative neoplasms; peptide antibodies

ZORA

Macrophage migration inhibitory factor (MIF) modulates trophic signaling through interaction with serine protease HTRA1

Author: Andersson Malin
Benedikz Eirikur
Elkjær Maria Louise
Fex Svenningsen Åsa
Hjæresen Simone
Holmskov Uffe
Huynh Ha Uyen Buu
Illes Zsolt
Löring Svenja
Martin Nellie
Moeller Jesper Bonnet
Nielsen Solveig Beck
Sørensen Anna Lahn
Publication venue: 'Springer Science and Business Media LLC'
Publication date: 01/01/2017
Field of study

Macrophage migration inhibitory factor (MIF), a small conserved protein, is abundant in the immune- and central nervous system (CNS). MIF has several receptors and binding partners that can modulate its action on a cellular level. It is upregulated in neurodegenerative diseases and cancer although its function is far from clear. Here, we report the finding of a new binding partner to MIF, the serine protease HTRA1. This enzyme cleaves several growth factors, extracellular matrix molecules and is implicated in some of the same diseases as MIF. We show that the function of the binding between MIF and HTRA1 is to inhibit the proteolytic activity of HTRA1, modulating the availability of molecules that can change cell growth and differentiation. MIF is therefore the first endogenous inhibitor ever found for HTRA1. It was found that both molecules were present in astrocytes and that the functional binding has the ability to modulate astrocytic activities important in development and disease of the CNS

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Publikationer från Uppsala Universitet

Digitala Vetenskapliga Arkivet - Academic Archive On-line

University of Southern Denmark Research Output