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Lecture 7 Viral vectors, continued… 19th November 2012 Adeno-associated viral vectors

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Page 1: Viral vectors, continued… - Jagiellonian Universitybiotka.mol.uj.edu.pl/zbm/handouts/2012/JD/gene_therapy/... · 2012-12-27 · Viral vectors, continued… 19th November 2012 Adeno-associated

Lecture 7

Viral vectors, continued…

19th November 2012

Adeno-associated viral vectors

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AAV

adenovirus

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Infectious cycle of AAV

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Adeno-associated viruses – AAV Small, non-pathogenic single stranded DNA viruses. There are at least 12 different serotypes of AAVs. The most common are AAv1 and AAV2 – 70-80% of human population is seropositive to this serotypes For replication require additional genes delivered by other viruses (adenoviruses or herpes simplex viruses) Genome AAV – 4681 nucleotides, at both ends there are 145 nt-long ITR (inverted terminal repeats) AAV infect both dividing and non-dividing cells Entering into the cells is dependent on binding to the receptor – different serotypes use various receptors AAV integrate into cellular geneome – in human this integrations is strictly specific, at chromosome 19 (AAVS1 – AAV integration site-1).

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removal of rap and cap genes transgene insertion

AAV vectors

ITR ITR

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6 Verma & Weitzman, Ann Rev Biochem 2005

Essential and non-essential elements in different viral vectors

ITR – necessary in cis – initiation of replication - packaging signal - integration into genome

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Scheme of the AAV genome

proteins

Rutkowski et al., Biotechnologia 2007

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Ways of production of AAV vectors

- dependent on helper vector

- helper-vectors independent

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Construction of AAV vectors – system with helper adenoviral

packaging cells

co-infection with adenovirus

recombinant AAV

adenovirus

capsid proteins

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Vectors in AAV helper-free system

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Helper-free production of AAV vectors (2)

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Strategies of production of AAV vectors

Rutkowski et al., Biotechnologia 2007

Packaging cells

Three vs two plasmid systems

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AAV and genomic integration

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Site-specific integration

• AAV integrates usually stably into a specific site on chromosome 19q13.3 (AAVS1)

• Integration region- AAVS1 (RBS,TRS) • Rep78 and Rep68 bind to a 109 bp

DNA fragment near AAVS1 and can mediate complex formation (DNA of chromosome 19 and AAV harpin DNA)

• Viral DNA replication within AAVS1 are likely involved in site-specific integration;

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AAV vectors features

- due to the lack of Rep68 and Rep78 the specific integration into chromosome 19 is lost

- unspecific integration (low efficacy, about 5-10%) - this unspecific integration preferentially occurs at the transcriptionally active genes. However, there is doubt whether the integration can be oncogenic - episomal expression

- however, because of non-immunogenic nature the episomal expression in non-dividing cells can be long-term

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How to deal with a small capacity of AAV vectors?

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AAV- concatamerisation

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AAV serotypes

12 serotypes are known

AAV-2 serotype is the most commonly used Different serotypes can employ various receptors to enter the cells - AAV-2: heparan sulphate - AAV-1 & AAV-5 – sialic acid - AAV-5 co-receptor: PDGF-B receptor

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AAV2 vector trafficking

Receptor – through heparan sulphate binding co-receptors: αVβ5, FGF receptor (FGF1r), c-met

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AAV vectors, in contrast to adenoviral, can provide long-term expression

Champion et al., Circulation 2003

Mouse heart

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Different transduction efficiency of AAV-2 viral vectors

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A C B

F E D

I H G

A C B

F E D

I H G

Transduction efficacy of AAV2 vectors depends on cell type

HEK 293

HeLa

HaCaT

Not transduced 1000 MOI 10 000 MOI

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C) mosaic capsid

19/1 3/1 1/1 1/3 1/19

Different ratios of plasmids

Rep1 Cap1 Rep2 Cap2

B) bi-specific antibody

cell-surface receptor (for e.g. endothelial cell)

A) transcapsidation

AAV9 5’

transgene

3’ AAV2

ITR

ITR Rep Cap

AAV2/9

D) chimeric capsid

5’

Rep Cap

3’

ITR

ITR

SIGYPLP

AAVsig

Methods enhancing the effectiveness of AAV vectors

Jazwa et al.,, Curr Gene Therapy, 2007

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Endothelial

Bronchial epithelial

Vascular smooth muscle

Skeletal muscle

Different transduction efficiency of AAV-2 viral vectors

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AAV cell entry via heparin sulfate

proteoglicans (HSPG) direct membrane

co-receptors:

avß5 integrin

FGFR1

Cell entry is independent on adenovirus presence. after B. J. Carter

HSPG

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GFP 587-SIGYPLP

pXX6

AAVsig Nicklin et al. Mol. Ther. 2001 vol. 4 (2)

Targeting of AAV vectors to endothelial cells

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HUVEC HSVEC

10,000 vector particles/cell

5.9-fold HUVEC 28.2-fold HSVEC

AAVsig wtAAV

Mol. Ther. 2001 vol. 4 (2)

Targeting of AAV vectors to endothelial cells

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Features of AAV vectors Advantages 1. Long term expression 2. High efficiency of transduction of many cell types 3. Non-pathogenic viruses. Low risk of cellular immune response, which is

additionaly limited by removal of viral sequences Limitations 1. Unspecific integration 2. Small capacity – max. 5 kbp 3. Low efficiency of transduction of certain cell types – targeting might be

required 4. Difficulty of production in sufficient titer for in vivo work 5. Risk of humoral immunity: antibodies detect capsid proteins

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AAV investigations on the new serotypes

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30 Su et al., Gene Therapy 2006

AAV1 provides earlier and higher expression in the heart than AAV2

1 day

14 days

14 days

Normal heart

Ischemic heart -expression in myocytes around the scar

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AAV8 provides higher expression in the rat heart

Palomeque et al.. Gene Therapy 2007

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AAV8 provides higher expression in the rat heart

Palomeque et al.. Gene Therapy 2007

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AAV9 is even more effective than AAV8 even at lower doses !

systemic delivery

Ianagaki et al., Mol Therapy 2006

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CA Pacak & BJ Byrne , Mol Ther 2011

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Self complementary AAV scAAV – short introduction

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Important rate-limiting step for transduction

scAAV created to improve transduction efficiency of AAV vectors

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RBE – Rep-binding element trs – terminal resolution site

!

Self complementary AAV

In scAAV one of the ITR sequences has been devoid of TRS (terminal resolution site), what eliminated the site of cutting for Rep protein (which has an activity of endonuclease). In this to the capsid is packed ds DNA

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Transduction efficiency of ssAAV and scAAV vectors in human fibroblast cells (10000 vetor particles/cell)

Han Z. et al. Mol Genet Metab. 2008 April 93(4): 381-387

Self complementary AAV

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Lead to enhanced formation of transcription-competent double-

stranded genomes

First publication: August 2001, McCarty DM et al.

Production and purification of scAAV vectors is the same as

conventional ssAAV

Demonstrated to be an improved transduction vector with a fast

onset of gene expression

Production of scAAV constructs with one mutated ITR typically yields > 90% dimeric genoms

Self complementary AAV

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scAAV vs ssAAV

Transgene expression evenly distributed among hepatocytes throughout the liver Transduce muscle cells 10 – 15 times more efficiently Greater saturation of transduced neuronal cells within limited area Transduce 2500-fold more retinal cells per particle at 5 weeks after infection Threefold increase in transduction after single infection in bone marrow-derived dendritic cells

There are, however, cell types that do not show improved transduction: polarized airway epithelial cell, primary B-cell chronic lypmhocytic leukemia cells Smaller capacity: only ~2,2 kb

Advantages Limitations

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Application of AAV in clinical gene therapy

1. Nervous system diseases – Canvan disease 2. Cystic fibrosis 3. Haemophilia – transfer of factor IX 4. Muscular dystrophy 5. Leber’s congenital amaurosis (blindness) 6. Cardiovascular diseases

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Other vectors

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HSV

Herpes simplex viruses

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Herpes virus – 1 Advantages

Very large genome – 152 kb – linear, double strand DNA, contains at least 84 genes, of which around half is not required for the virus replication

The virus itself is transmitted by direct contact and replicates in the skin or mucosal membranes before infecting cells of the CNS.

It exhibits both lytic and latent activity. The lytic cycle results in viral replication and cell death. The latent infection allows for the virus to be maintained in the host for an extended period of time.

The virus enters cells by fusion triggered by binding of viral glycoprotein gB and gD to the heparin sulfate moiety of the cell surface protein.DNAenters the cell and circularizes.

Large transgene can be introduced – up to 30 kb

Large number of viral copies can be produced

Virus is not toxic, may stay in latent form for a long time

Transduce numerous cell types Limitations Lack of data concerning the application of recombinant herpesviruses in patients Problems with targeting to specific cell type

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Applications of HSV-1 vectors

Experimental studies 1. Tumors, including nervous systems 2. Diseases of the central and peripheral nervous systems 3. Injury to spinal cord 4. Treatment of pain – delivery to sensory nerves looks particulalry promising

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Other viral vectors

1.retro-adenoviral vectors: contains LTR of retrovirus, capsid and other genome features of adenovirus 2. Polio virus, hepatitis A virus 3. Ebola virus lentiviral vectors containing proteins of Ebola virus capsid - infects cells of respiratory epithelium

4. Baculoviruses 5. Alpha viruses

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47 Nature Genetics,

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retroviruses

adenoviruses

AAV

naked DNA

liposomes

six years ago...

Types of vectors used in clinical trials of gene therapy