In constrast to demand for freshwater that increases continuously due to population growth and economic growth, the availability of freshwater resources decreases rapidly due to environmental pollution and climate change....
Rapid human papillomavirus (HPV) screening is urgently
needed for
preventing and early diagnosis of cervical cancer in rural areas.
To date, no HPV nucleic acid test (NAT) can be implemented within
a single patient visit starting from clinical samples. Here, we develop
a hydrogel loop-mediated isothermal amplification (LAMP) method in
a fashion of large-scale parallel (about 1000 cells) in situ HPV DNA
detection in clinical cervical exfoliated cells at the single-cell
level. It can be used with a hotplate and smartphone to obtain HPV
NAT results in less than 30 min, which is especially suitable for
the on-site scenario. We apply this rapid HPV NAT on 40 clinical cervical
exfoliated cell samples and compare the results to a clinical gold
standard quantitative polymerase chain reaction (qPCR) method [area
under curve (AUC), 1.00]. Meanwhile, our assay can provide HPV infection
information for large-scale parallel single clinical cervical exfoliated
cells, which cannot be received from traditional NAT methods. Our
findings suggest the potential of in situ hydrogel LAMP as a powerful
tool for clinical HPV screening and fundamental research.
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