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primerdimer

Primer-dimer is a common PCR artifact in which primers anneal to each other rather than to the target template, and are extended by the DNA polymerase to form short, non-target amplification products. It can occur in standard PCR, RT-PCR, and quantitative PCR (qPCR) assays and can interfere with amplification efficiency and detection.

Formation of primer-dimers arises when primers contain complementary regions, especially at their 3' ends, allowing them

The presence of primer-dimers can reduce yield of the intended product and, in qPCR, may contribute to

Prevention and mitigation strategies focus on primer design and reaction optimization. Avoid complementary sequences between primer

to
anneal
to
each
other
or
to
form
self-dimers.
If
the
3'
ends
are
aligned
in
a
way
that
permits
extension,
the
polymerase
can
copy
the
primer-primer
complex,
generating
short
double-stranded
fragments
typically
tens
of
base
pairs
long.
These
products
compete
with
the
desired
template
for
reagents
and
can
accumulate
during
cycling.
non-specific
fluorescence
signals
that
skew
Ct
values
and
complicate
data
interpretation.
In
conventional
PCR,
they
often
appear
as
faint,
small
bands
on
a
gel
or
appear
in
the
reaction
as
a
smear
near
the
bottom
of
the
gel.
pairs,
especially
at
3'
ends;
design
primers
with
balanced
Tm
and
minimal
potential
for
hairpins
or
dimers.
Use
primer
design
software,
validate
with
melt-curve
analysis,
and
employ
hot-start
polymerases
or
higher
annealing
temperatures.
Adjust
primer
concentrations,
Mg2+
levels,
or
switch
to
touchdown
PCR
if
necessary.
In
some
cases,
redesigning
primers
is
the
most
reliable
solution
to
eliminate
primer-dimers.