Engineering of a Lectibody Targeting High-Mannose-Type Glycans of the HIV Envelope

Hamorsky, Krystal Teasley; Kouokam, J. Calvin; Dent, Matthew; Grooms, Tiffany N.; Husk, Adam S.; Hume, Steven D.; Rogers, Kenneth A.; Villinger, François; Hanson, Carl V.; Matoba, Nobuyuki

doi:10.1016/j.ymthe.2019.07.021

Cited by 30 publications

(58 citation statements)

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“…The second ELISA utilized a mannosidase‐treated HIV gp120 (SF162, clade B). Given that Avaren likely binds to the terminal mannose residues of HMGs on the surface of gp120 (Hamorsky et al ., submitted; Matoba et al ., ), mannosidase treatment would eliminate Avaren's ability to bind gp120. On the contrary, VRC01 Fab binds to the CD4‐binding site and thus should bind gp120 regardless of mannosidase treatment.…”

Section: Resultsmentioning

confidence: 98%

“…This transgene contained the subtilisin‐like processing protease kex2p positioned between the heavy and light chains of the Fab whereby during expression the heavy and light chain would be translated as a single polypeptide followed by separation in the trans‐Golgi via cleavage by the kex2p protease. Once cleaved, the heavy and light chains would assemble into a functional Fab (Hamorsky et al ., ; submitted). The overexpressed VRC01 Fab ‐Avaren fusion was then extracted from the plants and purified using a three‐step chromatography procedure.…”

Section: Resultsmentioning

confidence: 99%

“…The yield may be improved by further optimization of expression and/or purification conditions, thereby making it more viable for scale up and manufacturing. The synergism displayed in the mixture of the bivalent parental molecules VRC01 IgG and Avaren‐Fc (Figure ), both of which we have previously produced in N. benthamiana (Matoba et al ., ; Hamorsky et al ., submitted), provided a rationale for, and strengthened our confidence in, utilizing these molecules in a fusion. To obtain a proof of concept, we opted for a simpler approach in this foundational study, creating a bispecific molecule monovalent for each antigen, VRC01 Fab ‐Avaren.…”

Section: Discussionmentioning

confidence: 94%

“…In this paper, we engineered a novel bispecific molecule based on the CD4 binding site‐specific bNAb VRC01 and the antiviral lectin Avaren, which showed superior potency compared to its parental proteins. The fusion protein, VRC01 Fab ‐Avaren, was expressed in N. benthamiana at approximately 40 mg/kg of leaf biomass, which was lower than those achieved for the parental molecules (~150 mg/kg for VRC01 (Matoba et al ., ; Hamorsky et al ., submitted), and over 100 mg/kg for Avaren). The yield may be improved by further optimization of expression and/or purification conditions, thereby making it more viable for scale up and manufacturing.…”

Section: Discussionmentioning

confidence: 95%

“…VRC01 Fab and Avaren were each purified by a two‐step purification scheme consisting of Talon Immobilized Metal Affinity Chromatography (IMAC) from Clontech followed by CHT chromatography from BioRad. Production of VRC01 and Avaren‐Fc were done as described previously (Hamorsky et al ., ; submitted).…”

Section: Methodsmentioning

confidence: 99%

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A novel anti‐HIV‐1 bispecific bNAb‐lectin fusion protein engineered in a plant‐based transient expression system

Kasinger

Dent

Mahajan

et al. 2019

Plant Biotechnology Journal

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Summary The discovery of broadly neutralizing antibodies (bNAbs) has been a major step towards better prophylactic and therapeutic agents against human immunodeficiency virus type 1 (HIV‐1). However, effective therapy will likely require a combination of anti‐HIV agents to avoid viral evasion. One possible solution to this problem is the creation of bispecific molecules that can concurrently target two vulnerable sites providing synergistic inhibitory effects. Here, we describe the production in plants and anti‐HIV activity of a novel bispecific fusion protein consisting of the antigen‐binding fragment (Fab) of the CD4 binding site‐specific bNAb VRC01 and the antiviral lectin Avaren, which targets the glycan shield of the HIV‐1 envelope (VRC01 Fab ‐Avaren). This combination was justified by a preliminary experiment demonstrating the synergistic HIV‐1 neutralization activity of VRC01 and Fc‐fused Avaren dimer (Avaren‐Fc). Using the GENEWARE ® tobacco mosaic virus vector, VRC01 Fab ‐Avaren was expressed in Nicotiana benthamiana and purified using a three‐step chromatography procedure. Surface plasmon resonance and ELISA demonstrated that both the Avaren and VRC01 Fab moieties retain their individual binding specificities. VRC01 Fab ‐Avaren demonstrated enhanced neutralizing activity against representative HIV‐1 strains from A, B and C clades, compared to equimolar combinations of VRC01 Fab and Avaren. Notably, VRC01 Fab ‐Avaren showed significantly stronger neutralizing effects than the bivalent parent molecules VRC01 IgG and Avaren‐Fc, with IC 50 values ranging from 48 to 310 p m . These results support the continued development of bispecific anti‐HIV proteins based on Avaren and bNAbs, to which plant‐based transient overexpression systems will provide an efficient protein engineering and production platform.

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Section: Resultsmentioning

confidence: 98%

Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 94%

Section: Discussionmentioning

confidence: 95%

Section: Methodsmentioning

confidence: 99%

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