Engineering chimeric antibodies aimed for passive mucosal

immunization against HRSV Shruti Bakshi1,2, Paloma Juarez1,2, Jorge Palaci1,2, Vikram Virdi1,2, Bert Schepens3,4, Xavier Saelens3,4 and Ann Depicker1,2

shruti.bakshi@psb.vib-ugent.be

1Department of Plant System Biology, VIB, Ghent, Belgium; 2Department of Plant Biotechnology and Bioinformatics, Ghent University, Belgium; 3Medical Biotechnology

Center, VIB, Ghent, Belgium; 4Department of Biomedical Molecular Biology, Ghent University, Belgium

Human Respiratory Syncytial Virus

Human Respiratory Syncytial Virus (HRSV) is the leading cause of acute lower respiratory tract infection in infants and frequently causes severe disease in the elderly. There is no licensed HRSV vaccine. As an alternative, the prophylactic treatment with an HRSV fusion protein targeting monoclonal antibody (mAb) is often recommended for infants that are at risk for developing HRSV infection. However, the high cost that is associated with the current mammalian cell-based mAb manufacturing systems hampers the broad implementation of this therapy. Also, it is possible that IgA type antibodies against HRSV may contribute even better to protection. Therefore, we aim to compare the effectiveness of IgG with secretory IgA based passive immunization against HRSV. In this context, we choose for the transient expression platform in plants that permits rapid small scale production of IgG and IgA based antibody versions [1].

Future Perspectives:

• Protein quantification to compare efficiency of our chimeric antibodies with commercially available antibodies.

• Fc effector function: In vivo (mouse models) comparisons will be done to test the effect of Fc tails. E4 antibodies (binding, but not neutralizing) will be useful for this purpose.

• Production of the most efficient neutralizing antibody in Arabidopsis seeds and challenge experiments in animal models.

Human IgG1

Fc

Mouse IgG2a

Fc

Mouse IgA

Fc

Mouse dIgA

Fc

Mouse sIgA

Fc

VHHC4

VHHD3

VHHE4

VHHV2

Monomeric Dimeric Secretory

Our Approach: We have genetically fused three different single domain antibodies [1] that are specific for the HRSV fusion protein F to the fragment crystallizable part (Fc) of different murine and human monomeric IgA and IgG antibodies. In order to obtain all different permutations we took advantage of the GoldenBraid2.0 [2] cloning system.

Since secretory IgA are the predominant antibodies in mucosal surfaces, they might be more effective than monomeric IgA and IgG in virus neutralization; therefore, IgA

based antibodies will also be tested in their dimeric and secretory forms.

A total of 15 different versions of chimeric antibodies against HRSV and 5 negative controls have been engineered and produced in Nicotiana benthamiana via Agrobacterium tumefaciens – mediated transient expression.

Synagis (50 µg/ml)

(Positive control)

VHH C4 + HuIgG1

VHH V2 + HuIgG1

(negative control)

Dilution Factor

Plaque reduction assay to assess the neutralization potency of RSV specific chimeric antibodies

Conclusions

• E4 nanobodies with the highest binding activity levels do

not neutralize RSV infection.

• A high binding activity of a given Nanobody® does not

translate to a high neutralizing activity.

a) Vacuum infiltration

b) Manual Infiltration

All the RSV specific antibodies showed binding activity for Fusion protein.

By means of combinatorial approaches using novel

synthetic biology tools, it is possible to transiently

express 20 different chimeric antibodies against RSV

in N. benthamiana,.

An

tI-F

pro

tein

Negative

control

1. Schepens, B., et al. (2011). "Nanobodies(R) specific for respiratory syncytial virus fusion protein protect against infection by inhibition of fusion." J Infect Dis 204(11): 1692-1701.

2. Sarrion-Perdigones, A., et al. (2011). "GoldenBraid: an iterative cloning system for standardized assembly of reusable genetic modules." PLoS ONE 6(7): e21622.

Monomeric Dimeric +

Monomeric

Secretory + Dimeric +

Monomeric

A B

C D E

Expression of the chimeric antibodies by agro-infiltration

in N. benthamiana plants

A B

C D E

0

0,1

0,2

0,3

0,4

0,5

0,6

0,7

10 100 1000 10000

OD

@ 4

92

nm

Dilution Factor

VHH + Human IgG1

C4-huIgG1

D3-HuIgG1

E4-HuIgG1

V2-HuIgG1

0

0,05

0,1

0,15

0,2

0,25

0,3

0,35

0,4

0,45

10 100 1000 10000

OD

@ 4

92

nm

Dilution Factor

VHH + Murine IgG2a

C4-MuIgG2a

D3-MuIgG2a

E4-MuIgG2a

V2-MuIgG2a

0

0,05

0,1

0,15

0,2

0,25

0,3

0,35

10 100 1000 10000

OD

@ 4

92

nm

Dilution Factor

VHH + Murine IgA (Monomeric)

C4-MuIgA

D3-MuIgA

E4-MuIgA

V2-MuIgA

0

0,05

0,1

0,15

0,2

0,25

0,3

0,35

10 100 1000 10000

OD

@ 4

92

nm

Dilution Factor

VHH + Murine IgA (Dimeric)

C4-MuIgA

D3-MuIgA

E4-MuIgA

V2-MuIgA

0

0,05

0,1

0,15

0,2

0,25

0,3

0,35

10 100 1000 10000

OD

@ 4

92

nm

Dilution Factor

VHH + Murine IgA (Secretory)

VHH C4

VHH D3

VHH E4

VHH V2

0

10

20

30

40

50

60

Nu

mb

er

of

Vir

us

Pla

qu

es

Dilution Factor

VHH-E4 chimeric antibody

E4-huIgG1

E4-muIgG2a

E4-muIgA

E4-muIgA (dimeric)

E4-muIgA (secretory)

Synagis (50 µg/ml)

PBS

0

10

20

30

40

50

60

Nu

mb

er

of

Vir

us

Pla

qu

es

Dilution Factor

VHH-D3 chimeric antibody

D3-huIgG1

D3-muIgG2a

D3-muIgA

D3-muIgA (dimeric)

D3-muIgA (secretory)

Synagis (50 µg/ml)

PBS

0

10

20

30

40

50

60

Nu

mb

er

of

Vir

us

Pla

qu

es

Dilution Factor

VHH-C4 chimeric antibody

C4-huIgG1

C4-muIgG2a

C4-muIgA

C4-muIgA (dimeric)

C4-muIgA (secretory)

Synagis (50 µg/ml)

PBS