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Ed. Note: The following
is a press release from Johns Hopkins Medical Institutions
September 4, 2005
-- An international team of researchers has discovered that human embryonic
stem cell lines accumulate changes in their genetic material over time.
The findings do
not limit the utility of the cells for some types of research or for some
future clinical applications, the researchers say, but draw attention to the
need to closely monitor stem cell lines for genetic changes and to study how
these alterations affect the cells' behavior. The researchers' work is
described in the Sept. 4 online edition of Nature Genetics.
"This is just the
first step," says Aravinda Chakravarti, Ph.D., one of the research team's
leaders and professor and director of the McKusick-Nathans Institute of
Genetic Medicine at Johns Hopkins. "While this is a snapshot of the genomic
changes that can happen, it's certainly not everything going on. We still
need comprehensive analyses of the changes and what they mean for the
functions of embryonic stem cells."
"Embryonic stem
cells are actually far more genetically stable than other stem cells, but
our work shows that even they can accumulate potentially deleterious changes
over time," adds Anirban Maitra, M.B.B.S., an assistant professor of
pathology at Johns Hopkins who shares first authorship of the paper with Dan
Arking, Ph.D., an instructor at Hopkins. Both are members of the
McKusick-Nathans Institute of Genetic Medicine at Johns Hopkins. "Now it
will be important to figure out why these changes occur, how they affect the
cells' behavior and how time affects other human embryonic stem cell lines."
The researchers
in the United States, Singapore, Canada and Sweden compared "early" and
"late" batches of each of nine federally approved human embryonic stem cell
lines. Twenty-nine human embryonic stem cell lines from seven different
companies are approved by the United States National Institutes of Health
under President George W. Bush's policy restricting federal funding of this
research to cell lines in existence before his announcement of the policy at
9 p.m. ET, Aug. 9, 2001. The dozens of human embryonic stem cell lines
developed since that announcement cannot be used in federally funded
research.
Most of the
"late" batches of stem cells -- those grown in the lab a year to three years
longer than their early counterparts -- displayed gross changes in the
number of copies of chromosomes or parts of chromosomes, in the marks that
control whether a gene is used by the cell, or in the sequence of DNA found
in the cell's mitochondria.
"The majority of
the lines we tested had genetic changes over time," says Chakravarti.
"Whenever you have something in a culture dish, it can change, and it will
be important to identify, keep track of and understand these changes."
At this point,
the precise effects of these changes on the cells aren't known, but some of
the changes resemble those seen in cancerous cells. At any rate, the changes
presumably became entrenched in a particular cell line because they
conferred some advantage as the cells were grown in laboratory dishes.
Whether the changes affect the stem cells' abilities to become other cell
types is also unknown.
Although research
with human embryonic stem cells is still in the lab -- not the clinic --
focusing on what the cells can do and how they are controlled, the hope is
that in the future these cells might help replace or repair tissues lost to
disease or injury. Because embryonic stem cells can become any type of cell
found in the body, in theory they could replace certain pancreas cells in
people with type I diabetes, or regenerate brain cells lost in a person with
Parkinson's disease, for example.
The analyses of
the embryonic stem cell lines and the computer comparisons of the mounds of
resulting data required the efforts of scientists at four academic centers,
two federal laboratories and three companies. Critical to the team's success
was prescient support of cutting-edge technology development by the National
Institutes of Health, support that enabled development of the technological
infrastructure necessary for large-scale comparative research, particularly
the Human Genome Project, says study co-author Mahendra Rao, M.B.B.S.,
Ph.D., of the Laboratory of Neurosciences at the National Institute on
Aging.
The scientists
used so-called GeneChip microarrays, or oligonucleotide arrays, to determine
whether there were genetic differences between the early and the late batch
of each of the stem cell lines, including whether any genes were present in
extra copies. Depending on the gene affected, extra copies could lead to
accelerated cell growth, increased cell death, or no measurable effect at
all.
In addition to
probing changes in the nuclear and mitochondrial DNA sequences and copy
numbers, the researchers examined whether the cells' genetic material had
shifts in marks that sit on genes and are passed from cell to cell during
cell division. These so-called epigenetic marks -- in this case methyl
groups on a gene region known as the promoter -- help control whether a gene
is used by a cell to make proteins. The researchers determined the
methylation status of 14 genes in each of the batches of stem cells; three
of the genes did show different methylation patterns in late batches
compared to early batches.
The scientists'
analysis revealed that five of the nine cell lines had extra or fewer copies
of at least one section of their genetic material in the late batch compared
to the same cell line's early batch. Two of the nine lines had changes in
their mitochondrial DNA over time, and all nine stem cell lines exhibited
some shift in methylation of at least one of three genes. One of these
genes, called RASSF1A, is also methylated in many cancers, but what effect
the methylation has on the stem cells is unknown.
The team is
already planning to conduct similar analyses of the remaining NIH-approved
cell lines, but analysis of stem cell lines not available for use with
federal funds will also be needed, the team members say.
The Johns Hopkins
researchers were funded by the Henry J. Knott Professorship in Genetic
Medicine, the Sol Goldman Pancreatic Cancer Research Center at Johns
Hopkins, the National Cancer Institute, the Maryland Cigarette Restitution
Fund and the Donald W. Reynolds Foundation Clinical Cardiovascular Research
Center at Johns Hopkins.
Authors on the
paper are Anirban Maitra, Dan Arking, Morna Ikeda, Keyaunoosh Kassauei,
Guoping Sui, David Cutler and Aravinda Chakravarti of Johns Hopkins; Narayan
Shivapurkar, Victor Stastny and Adi Gazdar of the University of Texas
Southwestern Medical Center; Ying Liu and Mahendra Rao of the National
Institute on Aging; Sandii Brimble and Thomas Schulz of BresaGen Inc.,
Athens, Ga.; Karin Noaksson, Johan Hyllner and Peter Sartipy of Cellartis
AB, Goteburg, Sweden; Xianmin Zeng and William Freed of the National
Institute on Drug Abuse; Alan Coleman of ES Cell International, Singapore;
Sei-Ichi Matsui of Roswell Park Cancer Institute and the State University of
New York at Buffalo; and Melissa Carpenter of Robarts Research Institute,
Ontario, Canada.
The microarrays
used in this work are the product of Affymetrix (Santa Clara, Calif.).
Chakravarti is a paid member of the Affymetrix scientific advisory board.
The terms of this arrangement are being managed by The Johns Hopkins
University in accordance with its conflict of interest policies.
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