Validation and in vivo characterization of research antibodies for Moesin, CD44, Midkine, and sFRP-1

Suzanne Doolen; Riham Ayoubi; Carl Laflamme; Ranjita Betarbet; Elizabeth Zoeller; Sean-Paul G Williams; Haian Fu; Allan I Levey; S J Sukoff Rizzo

doi:10.12688/f1000research.138354.2

Validation and in vivo characterization of research antibodies for Moesin, CD44, Midkine, and sFRP-1

F1000Res. 2024 Apr 23:12:1070. doi: 10.12688/f1000research.138354.2. eCollection 2023.

Authors

Suzanne Doolen¹, Riham Ayoubi², Carl Laflamme², Ranjita Betarbet^{3

4}, Elizabeth Zoeller⁴, Sean-Paul G Williams¹, Haian Fu^{4

5

6}, Allan I Levey^{7

8}, S J Sukoff Rizzo¹

Affiliations

¹ Aging Institute, University of Pittsburgh, Pittsburgh, Pennsylvania, 15219, USA.
² Neurology and Neurosurgery, McGill University, Montreal, Québec, H3A 2B4, Canada.
³ Center for Neurodegenerative Disease, Emory University, Atlanta, Georgia, 30322, USA.
⁴ Department of Pharmacology, Emory University, Atlanta, Georgia, 30322, USA.
⁵ Chemical Biology Discovery Center, Emory University, Atlanta, Georgia, 30322, USA.
⁶ Winship Cancer Institute, Emory University, Atlanta, Georgia, 30322, USA.
⁷ Neurology, Emory University, Atlanta, Georgia, 30322, USA.
⁸ Goizueta Alzheimer's Disease Research Center, Emory University, Atlanta, Georgia, USA.

Abstract

Background: A major goal of the Target Enablement to Accelerate Therapy Development for Alzheimer's disease (TREAT-AD) program is to develop and identify high-quality tools to test target or mechanistic hypotheses. As part of this initiative, it is important that commercial reagents including research antibodies being used to interrogate drug targets have confirmed validation data in knock-out cell lines. Ideally, these antibodies should also have utility for both in vitro and in vivo studies such that the levels of target proteins in target tissues can be quantified.

Methods: We evaluated commercial antibodies against TREAT-AD protein targets Moesin (Uniprot ID: P26038), CD44 (Uniprot ID: P16070), Midkine (Uniprot ID: P21741) and Secreted frizzled-related protein 1, referred to as "sFRP-1" (sFRP-1; Uniprot ID: Q8N474). Moesin, Midkine and sFRP-1, that were confirmed as selective based on data in knock-out cell lines. Western blot analysis was used to compare protein levels in brain homogenates from a mouse model with AD-relevant pathology (5XFAD) versus age-matched C57BL/6J control mice.

Results: Anti-Moesin ab52490 reacted in mouse brain homogenate with a predicted molecular weight of 68 kDa. Moesin protein expression was 2.8 times higher in 5xFAD compared to WT. Anti-CD44 ab189524 reacted with a band at the predicted size of 82 kDa. CD44 protein expression was 1.9 times higher in 5xFAD compared to WT. Anti-Midkine AF7769 reacted with a band ~16 kDa and a 17.8 times greater expression in 5xFAD compared to WT. Anti-sFRP-1 ab267466 reacted with a band at 35 kDa as predicted. sFRP-1 protein expression was 11.9 times greater in 5xFAD compared to WT.

Conclusions: These data confirm the utility of these selective commercially available antibodies against Moesin, CD44, Midkine, and sFRP-1 for in vivo studies in mice and provide insight into the use of 5XFAD mice for in vivo target engagement studies for these target proteins.

Keywords: 5xFAD; Midkine; Moesin; Western blot; antibody characterization; mice; sFRP-1; Alzheimer’s disease.

Publication types

Validation Study

MeSH terms

Alzheimer Disease / metabolism
Animals
Antibodies / immunology
Cytokines / metabolism
Humans
Hyaluronan Receptors* / immunology
Hyaluronan Receptors* / metabolism
Membrane Proteins / immunology
Membrane Proteins / metabolism
Mice
Microfilament Proteins* / immunology
Microfilament Proteins* / metabolism
Midkine* / metabolism

Substances

Midkine
Hyaluronan Receptors
moesin
Microfilament Proteins
Antibodies
Membrane Proteins
Cytokines

Grants and funding

This work was supported by the Emory-Sage-SGC TREAT-AD center established by the National Institutes of Aging (NIA) U54AG065187 grant and additional support by RF1AG057443 and by the Government of Canada through Genome Canada, Genome Quebec and Ontario Genomics (OGI-210). RA is supported by a Mitacs postdoctoral followship.