Heidi Ledford
|
Scientists
have created a biodegradable polymer that can shuttle DNA into cells,
raising the possibility that the compound may one day provide a safer
way of performing gene therapy.
There
have been more than 1,000 trials of gene therapy, a pioneering way of
fixing genetic defects by introducing new genetic material straight
into a person's DNA; most of these have been early stages of clinical
trials, to test for safety.
Most
of the trials rely on viruses to escort therapeutic fragments of DNA
through the gauntlet of cell membranes and myriad chemical landscapes
of the body, to insert it into a person's DNA. Safety concerns about
these viruses, including their potential to cause cancer, have made
nonviral approaches an attractive alternative.
Researchers
have tried several methods, from wrapping genes in positively charged
lipids to injecting pure, 'naked' DNA. None has achieved the efficiency
of a virus. "It's a hard thing to do to get DNA, which is this huge,
floppy, negatively charged molecule, from outside the body, through the
body, and then into the cell," says bioengineer Daniel Anderson of the
Massachusetts Institute of Technology in Cambridge. "There are a lot of
barriers."
Now
Anderson and his team have succeeded in using a polymer, known as a
poly(beta-amino ester), to successfully insert a gene into mouse
ovarian tumours, a process known as 'transfection'. In cell culture,
the new compound was able to transfect more than twice as many cells as
the leading nonviral reagent available.
The resulting level of gene expression rivalled that achieved by adenovirus, a commonly used gene-therapy vector.
"There
really hasn't been any nonviral system that can transfect human cells
this well," says Anderson. In this case, the inserted genetic
information simply made the mouse tumours express a fluorescent
protein. The same technique could, in theory, be used to deliver more
useful strings of DNA. That has yet to be trialled in live animals.
Success in the end
The
work follows on from earlier studies using positively charged polymers
that clump together with nucleic acid to form nanoparticles.
Previously, some of these polymers have been made to deliver their DNA
or RNA cargo to the inside of a cell. But they often work only for
short periods of time, and have to be used in concentrations that were
deemed too high for clinical use in humans.
Anderson
and his co-workers took a number of poly(beta-amino ester) polymer
backbones and gradually tweaked them, piece by piece, looking to
improve their efficacy. They created a library of variants by
chemically modifying the ends of the polymer, and looked for molecules
with improved transfection efficiency.
The
successful polymer had had both ends capped with a molecule called
primary diamine, increasing its ability to deliver DNA - possibly by
increasing the overall positive charge of the molecule. The results are
published in Advanced Materials.
Anderson says that his team will continue the work in animals, with an eye to moving to clinical trials in humans.
Transient expression
Although the results in cell culture are promising, it is
still unclear how well these polymers will function in live animals,
cautions biochemist Francis Szoka of the University of San Francisco in
California. "They still have a long way to go to show that it will be
useful for in vivo gene transfer," he says.
Specifically,
Szoka is concerned that the researchers only evaluated the activity of
the introduced genes in mice up to six hours after the polymer - DNA
combo was injected. Given that genes introduced by previous-generation
polymers had functioned only transiently, six hours of gene expression
is not enough to convince him that the same won't be true of Anderson's
modified poly(beta-amino ester), he says.
And,
although Anderson and his colleagues directly compared their polymer
with adenovirus in tissue culture, they did not perform a direct
comparison in live mice. Previous claims of success in cell culture
have not fared as well in animals. "So far nothing has been able to
translate into animals with good, high rates of transfection," says
Szoka.
Reference : Green, J.J., et al. Adv. Mater. doi: 10.1002/adma.200700371 (2007).
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