RICHMOND, Calif.,
Nov. 9, 2015 /PRNewswire/ --
Sangamo BioSciences, Inc.
(Nasdaq: SGMO), a leader in therapeutic genome editing, announced today the
publication in
Nature Biotechnology of data demonstrating efficient zinc
finger nuclease (ZFN)-mediated, targeted gene insertion in human hematopoietic
stem and progenitor cells (HSPCs). In addition, data published earlier this
month in
Nucleic Acids Research, demonstrate that similar
efficiencies can be obtained in primary human T-cells. Sangamo's genome editing
method provides a precisely targeted and therefore potentially safer approach
than traditional randomly integrative gene therapies, such as lentiviral
vectors, for the treatment of human diseases of the blood and immune system, and
the generation of T-cell based cancer immunotherapies.
"These studies present new and substantial data affirming that Sangamo's ZFN
genome-editing platform provides precise, robust targeted insertion of
therapeutic genes, in contrast to conventional integrating vector approaches,
such as lentiviral vectors that insert genes randomly," stated
Edward Lanphier, Sangamo's president, and chief
executive officer. "Our extensive clinical experience and a substantial body of
research, documents the accuracy and efficiency of our ZFN technology, and
positions it as a more versatile and potentially safer therapeutic strategy than
other gene therapy and genome editing approaches. Our technology also provides
an alternative manufacturing platform for cell therapies."
Researchers capitalized on the fact that ZFN-mediated genome editing requires
only transient expression of the ZFNs to effect a permanent change in the
genome. They used messenger RNA and electroporation to deliver the ZFNs and a
non-integrating vector, an adeno-associated virus (AAV) serotype 6, to provide a
therapeutic DNA sequence, a so-called "donor template", to HSPCs and CD4 and
CD8 T-cells. The "donor template" can encode an entire gene that integrates at
the targeted site of ZFN action. This delivery approach achieved efficiencies
of gene transfer and targeted integration of the therapeutic DNA sequence,
particularly in more primitive longer-lasting stem cells and T-cells, to levels
that can be used therapeutically to potentially treat a range of monogenic
diseases.
"Efficient targeted integration of a therapeutic gene into both hematopoietic
stem cells and T-cells represents a major step forward in the quest for more
precise and safer gene-based therapies," stated
Michael Holmes,
Ph.D., Sangamo's vice president, research, and a corresponding author on both
papers. "Importantly, in our hematopoietic stem cell work with our scientific
collaborators at
USC, we successfully modified a class of the most
pluripotent stem cells, leading to long-term production of ZFN-modified cells
across all blood cell lineages following transplantation into immune deficient
mice. Our results in these two studies provide a robust strategy for additional
therapeutic applications of ZFN-mediated genome editing in HSPCs and
T-cells."
The stem cell study,
"Homology-driven genome editing in hematopoietic stem
and progenitor cells using ZFN mRNA and AAV6 donors" was carried out in
collaboration with scientists in the laboratory of
Paula
Cannon, Ph.D., professor of molecular microbiology and immunology,
pediatrics, biochemistry and molecular biology, and stem cell biology and
regenerative medicine at the University of
Southern California, and was published as an
Advance Online Publication in
Nature Biotechnology.http://www.nature.com/articles/doi:10.1038/nbt.3408
The T-cell study,
"Highly efficient homology-driven genome editing in
human T-cells by combining zinc finger nuclease mRNA and AAV6 donor delivery"
was published as Advance Access in
Nucleic Acids Research
on
November 2, 2015.
http://nar.oxfordjournals.org/content/early/2015/11/01/nar.gkv1121.full.pdf+html
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