Rapid and sensitive detection of Mollicutes in cell culture by polymerase chain reaction

## Abstract Conventional reverse transcription‐polymerase chain reaction (RT‐PCR) to detect norovirus (NV) is a complex of multi‐step procedure that requires gel electrophoresis as well as hybridization or sequencing to confirm the final diagnosis. A duplex TaqMan RT‐PCR was developed to detect and

Several studies have been performed to assess the diagnostic value of using small tandem repeat (STR) markers and quantitative fluorescent polymerase chain reaction (QF-PCR) assays for the rapid detection of aneuploidies involving chromosomes

## Abstract Adenoviruses are associated with endemic and epidemic acute conjunctivitis, large nosocomial outbreaks reflecting virus transmission on unwashed hands or inadequately sterilised ophthalmic instruments. The polymerase chain reaction (PCR) proved more sensitive than antigen detection by i

Paraffin sections of 11 formalin-fixed trichilemthe genital HPVs (A); the epidermodysplasia verrucimomas were investigated for the presence of formis (EV)-associated HPVs (B); ungulate associated human papillomavirus (HPV) DNA by the polypapillomaviruses (C and D) and cutaneous HPVs (E) merase chain

germ cells, is not a good marker for CIS and seminoma of the testis.

## BACKGROUND. The sensitive detection of circulating tumor cells and micrometastases may have important therapeutic and prognostic implications. METHODS. The molecular detection of occult tumor cells can be accomplished by amplifying tumor specific abnormalities present in the DNA or mRNA of mali