34.9 ms (+ 9.7) and τ
150
u
= 55.7 ms (+ 16.3). Careful
selection and analysis of statistical models appropri-
ate for our data (with outliers always present) is part
of our ongoing work.
4 CONCLUSIONS
We have shown that single DNA hairpin molecules
captured in a biological nanopore can be detected and
reacted to using a finite state machine implemented
on a field-programmable gate array. The dwell time
of such translocation events can be extended to gain
more signal, which can in turn be analyzed offline
using machine learning methods to yield terminal
base-pair specific signatures. The signatures can then
be used for real-time identification of terminal base
pairs. Additionally, the finite state machine is ca-
pable of ejecting a molecule from the pore after it
has been detected but prior to unzipping the hair-
pin. Rapid DNA hairpin detection (< 2 msec) re-
lied on a mean filtered amplitude, which was required
to remain within a preset amplitude range (< 6 pA
in spread) for multiple consecutive threshold com-
parisons. The method will be tuned to differentiate
DNA-enzyme blockades from DNA alone blockades
in real time as part of our ongoing work. Ultimately,
nanopore-based characterization of enzyme dynamics
will require direct detection and control of multiple
DNA conformations relative to the enzyme, and direct
control of enzyme-free DNA is a prerequisite toward
developing this capability.
ACKNOWLEDGEMENTS
E. Koch was supported by a Summer Undergradu-
ate Research Fellowship in Information Technology,
funded by NSF under grant CCF-0552688. The work
was also supported in part by NHGRI under grant
K25 HG004035-01. We thank K. Lieberman and
M. Akeson for their help in preparing the paper.
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