Bispecific Antibody (BsAb) Design, Expression and Purification

Bispecific antibody (BsAb) is one kind of the next generation of antibody. The dual targeting is a particular concept linked with bsAbs, enabling them to target two different antigens on two different cells, two different antigens on the same cell, or two different epitopes on the same antigen.

According to the existence of the Fc (fragment crystallizable) region, bispecific antibodies can be divided into two categories: IgG-Based bsAbs and Fragment-Based bsAbs.

1. IgG-based bispecific antibody (BsAb)

IgG-Based bispecific antibodies are similar in structure to native antibodies, and all have Fc regions.

To prepare bsAbs in IgG format, two challenges should be met. One is heavy chain heterodimerization, in which that each heavy chain will only pair with the heavy chain of the second specificity. The second is cognate heavy chain and light chain paring, in which each heavy chain will only pair with the light chain of its own specificity.

1.1 IgG-like Bispecific Antibody CrossMAbCH1-CL

The CrossMAb technology is based on the crossover of the antibody domain within ONE Fab-arm of a bispecific IgG antibody to enable correct cognate heavy chain and light chain paring. The favorite format is CrossMAbCH1-CL, an engineered Fab carrying a CH1-CL domain crossover, without side products are formed. Whereas, the correct heavy chain heterodimerization can be enforced by mutation through the knobs into holes (KiH). This platform has proven to be one of the most versatile antibody engineering technologies, allowing the generation of various bispecific antibody formats, including bi-(1+1), tri- (2+1) and tetra-(2+2) valent bispecific antibodies, as well as non-Fc tandem antigen-binding fragment (Fab)-based antibodies. These asymmetric CrossMAbs can be produced using the well-established IgG production workstream based on one single standard Chinese hamster ovary cell line and typical upstream and downstream processing. The product is comparable in scale, yield, glycosylation, stability and quality to conventional IgG antibodies.

The molecular structure of CrossMab bispecific antibody (BsAb). Knob-into-hole (KiH) technique is used to achieve heavy chain heterodimerization, whereas, one correctly engineered Fab for cognate heavy chain and light chain paring is achieved by CH1-CL domain crossover, without side products are formed, and thus keeping one wild type Fab assembly correctly.
IgG-like CrossMab bispecific antibody (BsAb) design and production

1.2 IgG-like bispecific antibody Fab S-S Rebuilt®

Fusion Biolabs develop an optimized platform to meeting the correct both heavy chain heterodimerization through KiH (knobs into holes) and correct cognate heavy chain and light chain paring through our own Fab S-S Rebuilt technologies, in which an engineered disulfide bond between the antibodies’ variable domains that asymmetrically replaces the natural disulfide bond between CH1 and CL.

The molecular structure of Fab S-S-Rebuilt® bispecific antibody (BsAb). Knob-into-hole (KiH) technique is used to achieve heavy chain heterodimerization, and correct cognate heavy chain and light chain paring through Fab S-S Rebuilt technologies, in which an engineered disulfide bond between the antibodies’ variable domains that asymmetrically replaces the natural disulfide bond between CH1 and CL.
IgG-like Fab S-S-Rebuilt® bispecific antibody (BsAb) design and production

1.3 IgG4-like Bispecific Antibody (BsAb)

IgG4-like BsAb is a full length IgG-based BsAb. It is designed through KiH (heavy chain heterodimerization) and CH1-CL cognate heavy chain and light chain paring and interface through mutation replaced by T-cell receptor α/β constant domain to get bivalent IgG4 BsAb.

The molecular form of Ig4-like bispecific antibody (BsAb). Knob-into-hole (KiH) technique is used to achieve heavy chain heterodimerization, whereas, one correctly engineered Fab for cognate heavy chain and light chain paring is achieved by mutation of both CH1 and CL, and thus keeping one wild type Fab assembly correctly.
Ig4-like bispecific antibody (BsAb) design

1.4 IgG-like Tetravalent IgG-scFv BsAb

Both heavy chain heterodimerization and CH1-CL cognate heavy chain and light chain paring are meeting through DNA recombinant and cloning platform. IgG–scFv fusion, in which a scFv of one antigen specificity is fused to the c-terminal of a conventional IgG of a different antigen specificity. In construction of the IgG-scFv BsAb molecule, Fab A is first reformatted to a conventional IgG (Ab A). The VH and VL domains of Fab B are cloned and assembled into an scFv (scFv B) in the orientation, VH-(GGGGS)3-VL, and scFv B  is then fused to the c-terminal of Ab A  IgG CH3 domain. The IgG-scFv produced is purified by one- step Protein A affinity chromatography and retained high binding  affinity to both target A and target B.

IgG-scFv, a tetravalent IgG-like bispecific antibodies (BsAb), is constructed by a recombinant of a single-chain Fv (scFv) antibody fragment of one antigen specificity (scFvB) genetically fused to the C-terminal of a conventional IgG of a different antigen specificity (antigen A). Schematic diagram of the tetravalent IgG-scFv BsAb. The conventional IgG is from Fab A against target 1; the single-chain Fv (scFv) is from Fab B against target 2.
Schematic diagram of the tetravalent IgG-scFv bispecific antibody (BsAb)

1.5 IgG-like Dual-variable domain Ig (DVD-Ig) BsAb

Both heavy chain heterodimerization and CH1-CL cognate heavy chain and light chain paring are meeting through DNA recombinant and cloning platform. The DVD-Ig is designed as an IgG-like molecule, except that each light chain and heavy chain contains two variable domains in tandem through a short peptide linkage, instead of one variable domain. DVD-Igs are highly stable in vivo and exhibit excellent IgG-like physicochemical and pharmacokinetic properties.

The DVD-Ig is designed as an IgG-like molecule : DVD-Ig can be generated from two different monospecific mAbs. Both the light chain and heavy chain of a DVD-Ig have two variable domains (VL1, VL2 and VH1, VH2) fused in tandem through a short peptide linkage. The resulting DVD-Ig molecule retains the activities of both parental mAbs. With the appropriate peptide linkages between the two variable domains in both the heavy (VH1-VH2-CH) and light (VL1-VL2-CL) chains, the various motions within the Fab region (Fab elbow bend, Fab arm waving, rotation, etc.) can be maintained to provide sufficient structural freedom in the DVD-Ig to allow for dual binding.
Dual-variable domain Ig (DVD-Ig) bispecific antibodies (BsAb) design

2. Antibody fragment-based bispecific antibody (BsAb)

Fragment-based bsAbs are composed of the variable light and heavy domains from two antibodies, or the Fab units, and lack the Fc region which distinguishes them from IgG-Based bsAbs.

2.1 Bispecific diabodies, dimeric Single chain Diabodies (sc-diabodies) and tetrameric tandem diabodies (TandAb)

The procedure to design and make different disbodies are

1) Construction of genes encoding hybrid scFvs consisting of the VH  domain from one Ab A (VH A ) connected by a 5–10 amino acid linker to the V L  domain of another Ab B (VL B ) and the VH  domain from one Ab B (VH B ) connected by a 5–10 amino acid linker to the V L  domain of another Ab A(VLA );

2) Construction of a dicistronic operon for coexpression and co-secretion of two hybrid scFvs, VH A – VL B  and VH B – VLA , with the formation of functional heterodimer (diabody) in the bacterial periplasm to make bispecific Diabodies;

3) Joining the two dimerizing parts, VH A – VL B and VH B – VLA, with a peptide linker of 10–20 amino acids in length to make single chain-diabodies (scDb) or tandem diabodies (TandAb).

Cloning and design strategy for the generation of a bispecific diabody with the VH –VL configuration is shown. In the first step, the variable fragments of binding site A and site B (VHA or VHB and VLA or VLB) are amplified separately; then the variable domains of antibody A and antibody B are fused to create the structure VHA–V LB and VHB–VLA. In the last step, the two fragments are introduced into one expression vector combined to generate the bispecific diabody.
Bispecific diabody with the VH–VL configuration
Bispecific single-chain diabodies are generated by the expression of a single fragment of the format VHA–VLB–VHB–VLA (VH-VL configuration with 10-20 amino acid length middle linker) or of the format VLA–VHB–VLB–VHA (VL-VH configuration with 10-15 amino acid length middle linker). Generally, 10 amino acid short middle linker facilitate tandem diabodies (TandAbs), whereas, long middle linker facilitate single-chain diabodies (scDbs) formation.
Bispecific single-chain diabodies (scDb) and tetravalent tandem diabody (TandAb) design

2.2 Bispecific T cell engager (BiTE)

A recombinant antibody comprised of two tandem scFv, one binding CD3 on T cells, the other targeting a tumor antigen on tumor cells. BiTE constructs have the unique ability to engage any type of T-cell since the interaction does not involve co-stimulation or necessitate the involvement of a major histocompatibility complex.

Mechanism of action of bispecific T-cell engaging antibodies (BiTEs) consist of a single heavy and light chain of the variable region of a tumor-associated antigen (TAA), such as CD33 or CD123), and CD3 leading to the formation of a cytolytic synapse between T-cells and leukemic blasts. They are connected by a linker molecule, which defines the flexibility of the construct and antigen-binding kinetics in conjunction with the specific antigens used.
Bispecific T-cell engaging antibodies (BiTEs) structure and design

2.3 Bispecific dual-affinity Re-targeting molecules (DARTs)

DARTs are bispecific antibodies designed to simultaneously recognize both tumor antigens and invariant epitopes of the CD3/TCR complex on T cells. By doing so, they effectively recruit T lymphocytes to tumor targets in a noncognate fashion, bypassing the MHC context required for antigen recognition by the TCR. Theoretically, this enables all T cells to be redirected against the tumor. The DART (bispecific against B-cell C19 and T-cell CD3 structure) facilitates T-cell/B-cell associations, leading to potent redirected T cell–killing of B-cell lymphoma. DARTs generally are expressed in mammalian cell system CHO or HEK293.

Mechanism of action of basic construct of various bispecific antibodies (BsAbs) . Bispecific antibodies consist of a single heavy and light chain of the variable region of a tumor-associated antigen (TAA), such as CD33 or CD123; shown as black), and CD3 (illustrated as white) leading to the formation of a cytolytic synapse between T-cells and leukemic blasts. Dual-affinity re-targeting molecules (DARTs) , a scFv fragment based bispecific antibody format, have a similar basic structure but include a disulfide linker between VHA and VHB for additional stability.
Bispecific antibody: Dual-affinity re-targeting molecules (DARTs) design illustration

2.4 Bispecific tandem scFv: scFvA:scFvB

To making scFv based BsAb, scFv A and scFv B are separated by around a 25 amino acid flexible linker.

The tandem scFv fragment-based bispecific antibodies (BsAb) is constructed by two scFv (scFvA and scFvB) molecules connected through a short linker, which allows free rotation of the two separate folding and antigen-binding units, thus forming a very flexible structure (scFvA-scFvB).
Tandem scFv fragment-based bispecific antibodies (BsAb) design

Our services Provides two expression platforms:

1) E. coli bacterial expression system, which is seamlessly compatible with our phage display library constructionantibody phage panning and candidate validation projects.

2) Mammalian transient expression systems in CHO or HEK293 cells.

What We Offer: 

1. Antibody Fragment based BsAbs or IgG-based BsAbs design and produced from Synthetic DNA– This is the fastest route to construct BsAbs. Oligonucleotides are first assembled in vitro and then cloned into our in-house expression vectors.  The BsAb is then expressed in E. coli or a mammalian cell line. The turnaround time is 1-2 weeks. 

2. Antibody Fragment based BsAbs or IgG-based BsAbs design and produced from monoclonal cell line – VH and VL are obtained through the customer provided monoclonal hybridoma cells. The mRNA from the monoclonal will be cloned to create a cDNA vector from which the variable heavy (VH) and light (VL) chains are then subcloned into expression vector(s).

3. Antibody Fragment based BsAbs or IgG-based BsAbs design and produced from accession numbers – The VH and VL of the target monoclonal antibodies are synthesized according to the accession number, cloned, expressed, purified.

Key Features
  • Codon optimization technology
  • Seamless cloning technology
  • Two expression systems (either bacterial induction expression system or mammalia transient expression system)
  • Evaluation available, and scale-up option
Process Overview

 Client provides: Antibody sequence, plasmids containing coding sequence, or hybridoma cells (>1×10<sup>5</sup> cells, in liquid nitrogen or dry ice) with isotype or class information

Stage I: Variable Region (VH, VL) Sequencing or Gene Synthesis

Turnaround time: 5 days

Stage II: Bacterial expression vector or mammalian expression vector construction and sequence validation

Turnaround time: 5 days

Stage III: Transient expression or bacterial expression and affinity purification

Turnaround time: 1-2 weeks

Deliverables:

1) Purified BsAbs

2) Certificate of Analysis (COA) data sheet

Ordering Information

Antibody Fragment-based or IgG-based bispecific antibody design and production Services

CatalogDescriptionUnitPrice
82111Antibody fragment-based diabodies BsAds design and expression and affinity purification1 ProjectContact Us
82107Antibody fragment-based DARTs BsAds design and expression and affinity purification1 ProjectContact Us
82113Antibody fragment-based tandem scFv BsAbs design and expression and affinity purification1 ProjectContact Us
82108Antibody fragment-based BiTE BsAbs design and expression and affinity purification1 ProjectContact Us
82115IgG-based BsAbs design and expression and affinity purification1 ProjectContact Us

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