Detection of mammalian microRNA expression by in situ hybridization with RNA oligonucleotides

The original article included "100 mg/ml heparin" to describe the hybridization buffer, but it should correctly read "100 g/ml heparin." The corrected sentence is published in full below. The authors regret this error. "Hybridization buffer: 50% formamide, 0.3 mg/ml yeast RNA (ICN), 100 g/ml hepari

## Abstract Human rhinovirus 14 RNA was determined by in situ hybridization from middle turbinate biopsies in 32 patients with diagnosed common colds and in five control individuals. Twenty‐two (69%) biopsies from common colds patients but none of the five control biopsies showed reactivity for hum

## Abstract The value of biotinylated Oligonucleotide probes for screening and typing by in situ hybridization of the most frequent genital human papillomavirus infections (HPVs 6,11,16,18, 31, and 33) was assessed. Optimal hybridization conditions were defined on a panel of paraffin‐embedded tissu

## Abstract A rapid technique for the detection of hepatitis C virus (HCV) RNA in liver section using noniso‐topic in situ hybridization was described. Only 3 of the 10 patients seropositive for antibody to HCV and HCV RNA had detectable HCV RNA in the hepatocytes (1%, 2%, and 15% of cells positive

## Methods Mice DBM2 male mice were bred at the Walter and Eliza Hall Institute and were used when aged 6-8 weeks. Antibody The murine IgG2a monoclonal antibody F23.1 (Staerz et al., 1985) was purified from ascites by