| What's
New:
Naturally
occurring enzyme can break down key part of Alzheimer's
plaques
By
Michael Purdy
Oct.
24, 2006 -- Scientists have identified a naturally occurring
enzyme that can break down a key component of the brain
plaques characteristic of Alzheimer's disease. The finding
may provide researchers with new opportunities to understand
what goes wrong in the brains of Alzheimer's patients
and could one day help them seek new therapies.
Researchers
at Washington University School of Medicine in St. Louis
showed earlier this summer that the enzyme, matrix metalloproteinase
9 (MMP-9), degrades abnormally aggregated proteins known
as amyloid fibrils, a main ingredient of brain plaques.
In the brain, MMP-9 is made by support cells known as
astrocytes.
MMP-9
is already well-known because of its links to cancer
metastases, vascular disease, arthritis and other pathologies.
Scientists called the new link to Alzheimer's encouraging,
noting that previously identified enzymes only degrade
a smaller, nonaggregated component of Alzheimer's plaques.
"We
already knew of three enzymes that break down amyloid
beta (Abeta), a protein fragment that clumps together
with itself to form the fibrils," says Jin-Moo
Lee, M.D., Ph.D., assistant professor of neurology.
"But the thinking up until now had been that Abeta
might be clumping together so tightly that the fibrils
were indestructible."
In
a new study, appearing October 25 in The Journal of
Neuroscience, Lee's group found that disabling the mouse
gene for MMP-9 increased levels of Abeta in the spaces
between brain cells. The finding proves that MMP-9 contributes
to clearance of Abeta from extracellular spaces and
suggests its dysfunction could potentially contribute
to the development of Alzheimer's.
"MMP-9
and other enzymes like it are secreted from brain support
cells and active in the spaces outside of cells, and
that's where we saw an increase in Abeta levels in the
mice that lacked the gene for MMP-9," Lee notes.
"That's relevant to Alzheimer's because all the
amyloid plaques are extracellular, and the formation
of the plaques seems to be related to an elevated level
of Abeta that accumulates over time in those spaces."
In
earlier studies, Lee's lab analyzed the production of
MMP-9 in astrocytes. They found astrocytes close to
amyloid plaques increased their MMP-9 production. Imaging
studies also showed that MMP-9 levels increased around
blood vessels laden with amyloid.
"Astrocytes
become activated around plaques as they develop, and
then eventually form a wall surrounding the plaques,"
he says.
Lee's
results have led him to formulate a provocative but
as yet unproven theory about an old mystery of Alzheimer's
disease: why plaques continue to increase in number
over time but only grow to a certain size.
"Even
though everything we know about the fibrils suggests
they should constantly grow, plaques reach a mature
size and stop growing," Lee says. "It's possible
that production of MMP-9 and other similar substances
by support cells in the brain is establishing a balance
that prevents the plaques from growing beyond a certain
size."
To
follow up, Lee plans to crossbreed mice lacking MMP-9
with a line of mice genetically modified to develop
an Alzheimer's-like condition. Scientists want to see
if removing MMP-9 causes the mice to develop Alzheimer's
more quickly.
In
a parallel project that will test MMP-9's potential
as a therapeutic, Lee and his collaborators will use
viruses to alter production of MMP-9 in the mouse model.
Researchers want to learn if increasing levels of the
enzyme present in the brain can delay onset of Alzheimer's.
Yin
K-J, Cirrito JR, Yan P, Hu X, Xiao Q, Pan X, Bateman
R, Song H, Hsu F-F, Turk J, Xu J, Hsu CY, Mills JC,
Holtzman DM, Lee J-M. Matrix metalloproteinases expressed
by astrocytes mediate extracellular amyloid-beta peptide
catabolism. The Journal of Neuroscience, Oct. 25, 2006.
Yan
P, Hu X, Song H, Yin K, Bateman RJ, Cirrito JR, Xiao
Q, Hsu F-F, Turk JW, Xu J, Hsu CY, Holtzman DM, Lee
JM. Matrix metalloproteinase-9 degrades amyloid-beta
fibrils in vitro and compact plaques in situ. The Journal
of Biological Chemistry, June 20, 2006.
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