Aggregates in blood filter chambers used from the plasma donations of anti-D donors: evaluation for monoclonal antibody discovery using phage display.

McGowan, EC; Flower, RL; Jones, ML; Irving, DO; Barnard, RT; Hyland, CA; Mahler, SM; Bui, XT

Aggregates in blood filter chambers used from the plasma donations of anti-D donors: evaluation for monoclonal antibody discovery using phage display.

McGowan, EC Flower, RL Jones, ML Irving, DO Barnard, RT Hyland, CA Mahler, SM Bui, XT

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Publisher:: SIMTI Servizi srl
Publication Type:: Journal Article
Citation:: Blood Transfusion, 2021, 19, (1), pp. 64-72
Issue Date:: 2021-01

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Field	Value	Language
dc.contributor.author	McGowan, EC
dc.contributor.author	Flower, RL
dc.contributor.author	Jones, ML
dc.contributor.author	Irving, DO
dc.contributor.author	Barnard, RT
dc.contributor.author	Hyland, CA
dc.contributor.author	Mahler, SM
dc.contributor.author	Bui, XT
dc.date.accessioned	2022-07-03T22:02:44Z
dc.date.available	2020-07-17
dc.date.available	2022-07-03T22:02:44Z
dc.date.issued	2021-01
dc.identifier.citation	Blood Transfusion, 2021, 19, (1), pp. 64-72
dc.identifier.issn	1723-2007
dc.identifier.issn	2385-2070
dc.identifier.uri	http://hdl.handle.net/10453/158576
dc.description.abstract	BACKGROUND: RhD-immunoglobulin (RhIg) prevents anti-D alloimmunisation in D-negative pregnant women when the fetus is D-positive, reducing the incidence of haemolytic disease of the fetus and newborn. Manufacturing RhIg is reliant on the limited supply of plasma donations with anti-D antibodies. Monoclonal antibody (mAb) development platforms such as phage display, require blood samples to be collected from anti-D donors, which may be a complicated process. The blood filter chamber (BFC) discarded after an anti-D donor's donation might provide a source of Ig-encoding RNA. This study aims to evaluate whether used BFCs are a suitable source of Ig-encoding RNA for phage display. MATERIAL AND METHODS: Haemonetics PCS2 BFCs were obtained from 10 anti-D donors for total RNA extraction, cDNA synthesis and amplification of VH and VL IgG sequences for assembly of single-chain variable fragments (scFvs). A scFv-phage display library was constructed and 3 rounds of biopanning were performed using D-positive and D-negative red blood cells (RBCs). Positive phage clones were isolated, Sanger sequenced and, where possible, reformatted into full-length human IgGs to define specificity. The BFC aggregates from 2 anti-D donors underwent a Wright-Giemsa stain and hematological cell count. RESULTS: Of 10 BFCs, a sufficient yield of total RNA for library construction was obtained from BFCs containing cellular aggregates (n=5). Aggregate analysis showed lymphocytes were the cellular source of Ig-encoding RNA. From the 5 samples with aggregates, scFvs were assembled from amplified IgG variable regions. The library constructed from 1 of these samples resulted in the isolation of clones binding to D-positive RBCs with IGHV3 gene usage. Of the 4 reformatted IgG, 3 were anti-D and 1 had undefined specificity. DISCUSSION: BFC aggregates are a new and convenient source of Ig-encoding RNA which can be used to construct Ig gene libraries for mAb isolation and discovery via antibody phage display.
dc.format	Print-Electronic
dc.language	eng
dc.publisher	SIMTI Servizi srl
dc.relation.ispartof	Blood Transfusion
dc.relation.isbasedon	10.2450/2020.0093-20
dc.rights	info:eu-repo/semantics/openAccess
dc.subject	1102 Cardiorespiratory Medicine and Haematology
dc.subject.mesh	Animals
dc.subject.mesh	Antibodies, Monoclonal
dc.subject.mesh	Blood Donors
dc.subject.mesh	CHO Cells
dc.subject.mesh	Cricetulus
dc.subject.mesh	Filtration
dc.subject.mesh	Gene Library
dc.subject.mesh	Humans
dc.subject.mesh	Peptide Library
dc.subject.mesh	Plasma
dc.subject.mesh	Rho(D) Immune Globulin
dc.subject.mesh	RNA
dc.subject.mesh	Animals
dc.subject.mesh	Antibodies, Monoclonal
dc.subject.mesh	Blood Donors
dc.subject.mesh	CHO Cells
dc.subject.mesh	Cricetulus
dc.subject.mesh	Filtration
dc.subject.mesh	Gene Library
dc.subject.mesh	Humans
dc.subject.mesh	Peptide Library
dc.subject.mesh	Plasma
dc.subject.mesh	RNA
dc.subject.mesh	Rho(D) Immune Globulin
dc.title	Aggregates in blood filter chambers used from the plasma donations of anti-D donors: evaluation for monoclonal antibody discovery using phage display.
dc.type	Journal Article
utslib.citation.volume	19
utslib.location.activity	Italy
utslib.for	1102 Cardiorespiratory Medicine and Haematology
pubs.organisational-group	/University of Technology Sydney
pubs.organisational-group	/University of Technology Sydney/Faculty of Health
pubs.organisational-group	/University of Technology Sydney/Faculty of Health/Public Health
utslib.copyright.status	open_access	*
pubs.consider-herdc	false
dc.date.updated	2022-07-03T22:02:43Z
pubs.issue	1
pubs.publication-status	Published
pubs.volume	19
utslib.citation.issue	1

Abstract:

BACKGROUND: RhD-immunoglobulin (RhIg) prevents anti-D alloimmunisation in D-negative pregnant women when the fetus is D-positive, reducing the incidence of haemolytic disease of the fetus and newborn. Manufacturing RhIg is reliant on the limited supply of plasma donations with anti-D antibodies. Monoclonal antibody (mAb) development platforms such as phage display, require blood samples to be collected from anti-D donors, which may be a complicated process. The blood filter chamber (BFC) discarded after an anti-D donor's donation might provide a source of Ig-encoding RNA. This study aims to evaluate whether used BFCs are a suitable source of Ig-encoding RNA for phage display. MATERIAL AND METHODS: Haemonetics PCS2 BFCs were obtained from 10 anti-D donors for total RNA extraction, cDNA synthesis and amplification of VH and VL IgG sequences for assembly of single-chain variable fragments (scFvs). A scFv-phage display library was constructed and 3 rounds of biopanning were performed using D-positive and D-negative red blood cells (RBCs). Positive phage clones were isolated, Sanger sequenced and, where possible, reformatted into full-length human IgGs to define specificity. The BFC aggregates from 2 anti-D donors underwent a Wright-Giemsa stain and hematological cell count. RESULTS: Of 10 BFCs, a sufficient yield of total RNA for library construction was obtained from BFCs containing cellular aggregates (n=5). Aggregate analysis showed lymphocytes were the cellular source of Ig-encoding RNA. From the 5 samples with aggregates, scFvs were assembled from amplified IgG variable regions. The library constructed from 1 of these samples resulted in the isolation of clones binding to D-positive RBCs with IGHV3 gene usage. Of the 4 reformatted IgG, 3 were anti-D and 1 had undefined specificity. DISCUSSION: BFC aggregates are a new and convenient source of Ig-encoding RNA which can be used to construct Ig gene libraries for mAb isolation and discovery via antibody phage display.

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http://hdl.handle.net/10453/158576