bioRxiv (Cold Spring Harbor Laboratory),
Год журнала:
2024,
Номер
unknown
Опубликована: Май 14, 2024
Chikungunya
(CHIKV),
o'nyong-nyong
(ONNV),
and
Mayaro
(MAYV)
viruses
are
transmitted
by
mosquitoes
known
to
cause
a
debilitating
arthritogenic
syndrome.
These
alphaviruses
have
emerged
re-emerged,
leading
outbreaks
in
tropical
subtropical
regions
of
Asia,
South
America,
Africa.
Despite
their
prevalence,
there
persists
critical
gap
the
availability
sensitive
virus-specific
point-of-care
(POC)
diagnostics.
Traditional
immunoglobulin-based
tests
such
as
enzyme-linked
immunosorbent
assay
(ELISAs)
often
yield
cross-reactive
results
due
close
genetic
relationship
between
these
viruses.
Molecular
diagnostics
quantitative
polymerase
chain
reaction
(qPCR)
offer
high
sensitivity
but
limited
need
for
specialized
laboratory
equipment.
Recombinase
amplification
(RPA),
an
isothermal
method,
is
promising
alternative
qPCR,
providing
rapid
with
minimal
equipment
requirements.
Here,
we
report
development
validation
three
RPA-based
POC
CHIKV,
ONNV,
MAYV.
demonstrated
both
speed
sensitivity,
capable
detecting
10
viral
copies
within
20
minutes
amplification,
without
exhibiting
cross-reactivity.
Furthermore,
evaluated
clinical
potential
using
serum
tissue
samples
from
MAYV-infected
mice,
well
CHIKV-infected
human
patients.
We
demonstrate
that
RPA
amplicons
derived
patient
can
be
sequenced,
enabling
cost-effective
molecular
epidemiological
studies.
Our
findings
highlight
significance
specific
improving
early
detection
management
arboviral
infections.
bioRxiv (Cold Spring Harbor Laboratory),
Год журнала:
2025,
Номер
unknown
Опубликована: Янв. 21, 2025
Abstract
La
Crosse
virus
(LACV)
is
a
mosquito-borne
arbovirus
that
causes
pediatric
encephalitis
in
North
America,
primarily
affecting
children
under
the
age
of
16
years
age.
Early
and
accurate
diagnosis
crucial
to
reducing
morbidity
this
vulnerable
population;
however,
existing
molecular
serological
methods
face
limitations
sensitivity,
specificity,
accessibility.
Here,
we
present
development
reverse
transcription
recombinase
polymerase
amplification
(RT-RPA)
assay
for
LACV
detection.
Our
detects
within
20
minutes
with
limit
detection
100-1000
viral
copies,
demonstrating
high
specificity
without
cross-reactivity
against
closely
related
or
geographically
relevant
arboviruses.
We
further
integrate
RT-RPA
into
lateral
flow
format,
potentially
enabling
simple
inexpensive
point-of-care
diagnosis.
To
complement
our
development,
investigated
pathogenesis
mouse
model
recapitulates
age-dependent
susceptibility
observed
human
populations.
Using
assay,
reveal
invades
brains
weanling
mice
as
early
4
days
post-infection
(dpi)
adult
by
5
dpi.
Surviving
had
no
detectable
their
These
results
underscore
utility
RT-RPA-based
platform
offer
novel
insights
temporal
dynamics
neuroinvasion
clearance.
Scientific Reports,
Год журнала:
2024,
Номер
14(1)
Опубликована: Дек. 3, 2024
Chikungunya
(CHIKV),
o'nyong-nyong
(ONNV),
and
Mayaro
(MAYV)
viruses
are
transmitted
by
mosquitoes
known
to
cause
a
debilitating
arthritogenic
syndrome.
These
alphaviruses
have
emerged
re-emerged,
leading
outbreaks
in
tropical
subtropical
regions
of
Asia,
South
America,
Africa.
Despite
their
prevalence,
there
persists
critical
gap
the
availability
sensitive
virus-specific
point-of-care
(POC)
diagnostics.
Traditional
immunoglobulin-based
tests
such
as
enzyme-linked
immunosorbent
assay
(ELISA)
often
yield
cross-reactive
results
due
close
genetic
relationship
between
these
viruses.
Molecular
diagnostics
quantitative
polymerase
chain
reaction
(qPCR)
offer
high
sensitivity
but
limited
need
for
specialized
laboratory
equipment.
Recombinase
amplification
(RPA),
an
isothermal
method,
is
promising
alternative
qPCR,
providing
rapid
with
minimal
equipment
requirements.
Here,
we
report
development
validation
three
RT-RPA-based
CHIKV,
ONNV,
MAYV.
demonstrated
both
speed
sensitivity,
capable
detecting
10–100
viral
copies
within
20
min
amplification,
without
exhibiting
cross-reactivity.
Furthermore,
evaluated
clinical
potential
using
serum
tissue
samples
from
MAYV-infected
mice,
well
CHIKV-infected
human
patients.
We
demonstrate
that
RPA
amplicons
derived
patient
can
be
sequenced,
enabling
cost-effective
molecular
epidemiological
studies.
Our
findings
highlight
significance
specific
improving
early
detection
management
arboviral
infections,
particularly
resource-limited
settings.
Biomedicines,
Год журнала:
2023,
Номер
11(2), С. 610 - 610
Опубликована: Фев. 18, 2023
The
emergence
of
the
new
pathogen
SARS-CoV-2
determined
a
rapid
need
for
monoclonal
antibodies
(mAbs)
to
detect
virus
in
biological
fluids
as
tool
identify
infected
individuals
be
treated
or
quarantined.
majority
commercially
available
antigenic
tests
rely
on
detection
N
antigen
biologic
fluid
using
anti-N
antibodies,
and
their
capacity
specifically
subjects
by
is
questionable
due
several
structural
analogies
among
proteins
different
coronaviruses.
In
order
produce
specific
BALB/c
mice
were
immunized
three
times
at
20-day
intervals
with
recombinant
spike
(S)
protein.
procedure
used
was
highly
efficient,
40
mAbs
isolated,
purified
characterized,
13
ultimately
being
selected
specificity
lack
cross
reactivity
other
human
epitopes
recognized
identified
through
peptide
library
and/or
fragments
S
particular,
linear
along
S1,
excluding
receptor
binding
domain,
S2
subunits
protein
its
major
variants
concern.
We
combinations
anti-S
suitable
use
ELISA
diagnostic
tests,
highest
sensitivity
coming
from
proof-of-concept
antigens,
individuals,
that
represent
important
additional
tools
diagnosis
COVID-19.
Travel Medicine and Infectious Disease,
Год журнала:
2023,
Номер
52, С. 102548 - 102548
Опубликована: Фев. 9, 2023
We
aim
to
determine
if
nasal
samples
have
equivalent
detection
sensitivity
nasopharyngeal
swabs
for
RAT
and
evaluate
the
diagnostic
accuracy
of
with
RAT.
JBI Evidence Synthesis,
Год журнала:
2024,
Номер
22(10), С. 1939 - 2002
Опубликована: Авг. 26, 2024
The
objective
of
this
review
was
to
determine
the
diagnostic
accuracy
currently
available
and
upcoming
point-of-care
rapid
antigen
tests
(RATs)
used
in
primary
care
settings
relative
viral
genetic
real-time
reverse
transcriptase
polymerase
chain
reaction
(RT-PCR)
test
as
a
reference
for
diagnosing
COVID-19/SARS-CoV-2
adults.
Naval Research Logistics (NRL),
Год журнала:
2023,
Номер
71(1), С. 87 - 108
Опубликована: Авг. 3, 2023
Abstract
We
study
the
problem
of
designing
optimal
targeted
mass
screening
non‐uniform
populations.
Mass
is
an
essential
tool
that
widely
utilized
in
a
variety
settings,
for
example,
preventing
infertility
through
programs
sexually
transmitted
diseases,
ensuring
safe
blood
supply
transfusion,
and
mitigating
transmission
infectious
diseases.
The
objective
to
maximize
overall
classification
accuracy
under
limited
budget.
In
this
paper,
we
address
by
proposing
proactive
optimization‐based
framework
factors
population
heterogeneity,
budget,
different
testing
schemes,
availability
multiple
assays,
imperfect
assays.
By
analyzing
resulting
optimization
problem,
take
advantage
structure
as
multi‐dimensional
fractional
knapsack
identify
efficient
globally
convergent
threshold‐style
solution
scheme
fully
characterizes
across
entire
budget
spectrum.
Using
real‐world
data,
conduct
geographic‐based
nationwide
case
on
COVID‐19
United
States.
Our
results
reveal
identified
strategies
substantially
outperform
conventional
practices
significantly
lowering
misclassifications
while
utilizing
same
amount
Moreover,
our
provide
valuable
managerial
insights
with
regard
distribution
geographic
regions.
