Credit:
MRC Laboratory of Medical Sciences, MRC Laboratory for Molecular Biology
A
collaboration between researchers at the Laboratory of Medical Sciences (LMS)
in London and the Laboratory of Molecular Biology (LMB) in Cambridge, has
solved a decades-old mystery which could pave the way to better cancer
treatments in the future.
The work, which uncovered the basic
mechanism of how one of our most vital DNA repair systems recognizes DNA
damages and initiates their repair, has eluded researchers for many years.
Using cutting edge imaging techniques to visualize how these DNA repair
proteins move on a single molecule of DNA, and electron microscopy to capture how they "lock-on" to
specific DNA structures, this research opens the way to more effective cancer
treatments.
The collaboration between the
laboratories of Professor David Rueda (LMS) and Dr. Lori Passmore (LMB) has
been a brilliant example of how #teamscience can bear fruitful results and
underscores the importance of these two institutes in driving forward research
that unlocks the fundamental mechanisms of biology which will underpin the
future translation of that work into improvements in human health.
The researchers were working on a DNA
repair pathway, known as the Fanconi Anemia [FA] pathway, which was identified
more than 20 years ago.
DNA is constantly damaged throughout our
lives by environmental factors including UV light from the sun, alcohol use,
smoking, pollution and exposure to chemicals. One way in which DNA becomes
damaged is when it is "cross-linked," which stops it being able to
replicate and express genes normally.
In order to replicate itself and to read and express genes, the two strands of the DNA double helix first has to unzip into single strands. When DNA is cross-linked, the "nucleotides" (the "steps" in the double-helix ladder of DNA) of the two strands become stuck together, preventing this unzipping.
A single molecule of DNA (not directly visible)
is captured using microscopic beads (the large circles). Each of the red, green
or yellow dots moving between the beads represent a FANCD2I-FANCI protein
complex sliding along the DNA molecule, monitoring it for damage. Credit: MRC
Laboratory of Medical Sciences
The accumulation of DNA damages
including cross-linking can lead to cancer. The FA pathway is active throughout
our lives and identifies these damages and repairs them on an ongoing basis.
Individuals who have mutations that
make this pathway less effective are far more susceptible to cancers. Although
the proteins involved in the FA pathway were discovered some time ago, a
mystery remained over how they identified the cross-linked DNA and started the
process of DNA repair.
The team from the MRC LMS sister
institution, the LMB in Cambridge, led by Lori Passmore, had previously
identified that the FANCD2-FANCI (D2-I) protein complex, which acts in one of
the first steps of the FA pathway, clamps onto DNA, thereby initiating DNA
repair at crosslinks.
However, key questions remained:
how does D2-I recognize crosslinked DNA, and why is the D2-I complex also
implicated in other types of DNA damage?
The research, published in Nature, used a combination of
cutting-edge scientific techniques to show that the D2-I complex slides along
the double-stranded DNA, monitoring its integrity, and has also elegantly
visualized how it recognizes where to stop, allowing the proteins to move and lock
together at that point to initiate DNA repair.
Artur Kaczmarczyk and Korak Ray in
David Rueda's Single Molecule Imaging group, working with Pablo Alcón in Lori
Passmore's group, used a state-of-the-art microscopy technique known as
"correlated optical tweezers and fluorescence imaging" to explore how
the D2-I complex slides along a double-stranded DNA molecule.
Using optical tweezers, they could
catch a single DNA molecule between two beads, which allowed them to precisely
manipulate the DNA and incubate it with chosen proteins.
Using fluorescently labeled D2-I and single-molecule imaging, they observed how individual D2-I complexes bind to and slide along DNA, scanning the double helix. They discovered that rather than recognizing the crosslink between the two strands of DNA directly, the FA clamp instead stops sliding when it reaches a single-stranded DNA gap, a region where one of the two strands of DNA is missing.
The video shows the FANCD2-FANCI complex clamping
to DNA in order to repair it. Credit: MRC Laboratory of Medical Sciences, MRC
Laboratory for Molecular Biology
Using cryo-electron microscopy, a
powerful technique which can visualize proteins at a molecular level, the
researchers next determined the structures of the D2-I complex both in its
sliding position and stalled at the junction between single-stranded and
double-stranded DNA.
This revealed that the contacts
D2-I makes with this single-stranded–double-stranded DNA junction is distinct
from the contacts it makes with double-stranded DNA alone.
This allowed them to identify a
specific portion of the FANCD2 protein, called the "KR helix" that
they showed in their single-molecule imaging experiments is critical for
recognizing and stalling at the single-stranded DNA gaps.
Working with Guillaume Guilbaud and
Julian Sale in the LMB's PNAC Division, and Themos Liolios and Puck Knipscheer
at the Hubrecht Institute, Netherlands, they further showed that the D2-I
complex's ability to stall at these junctions using the KR helix is critical
for DNA repair by the FA pathway.
When DNA normally replicates in our
cells, it unzips the two DNA strands and copies each single strand. This creates a 'replication
fork' where the original DNA strands are unwound and new
double-stranded DNA is formed on each strand. However, when this fork reaches a
DNA crosslink, the strands cannot be unzipped, stalling the usual DNA
replication process.
This stalled
replication fork thus contains exposed single-stranded gaps where the DNA has
been unwound but not replicated. This research has shown that it is these
junctions between single- and double-stranded DNA at the stalled replication
fork that the D2-I protein complex latches tightly onto.
Not only does
this allow D2-I complex to bring other FA pathway proteins to the DNA crosslink
to initiate repair, but it also anchors the remaining double-stranded DNA,
protecting the stalled "replication fork" from enzymes in the cell
that would chew up the exposed end of the DNA strand and further damage the
DNA.
This work has
shown that it is DNA structures within the replication fork that stalls as a
result of cross-linked DNA, rather than the cross-linked DNA itself, that
triggers the D2-I complex to stop sliding and clamp on to DNA to initiate
repair. These stalled replication forks appear in many types of DNA damage,
explaining the broad role of the D2-I complex in other forms of DNA repair as
well as via the FA pathway.
Understanding
the process of DNA repair, and, importantly, why it fails, holds huge
importance as DNA damage is a key factor in many diseases. Critically, many
cancer drugs, for example Cisplatin, work by inducing such serious cellular
damage to cancer cells that they stop dividing and die.
In such cases, DNA repair pathways—such a vital physiological process in normal life—can be hijacked by cancer cells who use them to resist the effects of chemotherapy drugs. Understanding the mechanistic basis of the first step in the DNA repair pathway may lead to ways of sensitizing patients so that cancer drugs can be more effective in future.
by Medical Research Council (MRC) Laboratory of Medical Sciences
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