FIBROPAPILLOMATOSIS (FP) of sea turtles is a debilitating disease which is characterised by multiple benign cutaneous fibropapillomas and occasional visceral fibromas (Herbst 1994). Fibroepithelial tumours, which are commonly found on the turtles' conjunctivae and skin, interfere with vision, feeding and locomotion, and visceral nodules can fatally disrupt normal organ function (Herbst 1994, Herbst and others 1999). The aetiology of FP is unproven, but the disease has been experimentally induced in tumour-free turtles in captivity by inoculation of cell-free filtrates of tumour homogenates, consistent with a viral aetiology (Herbst and others 1995). The transforming agent is chloroform-sensitive, which suggests that if the agent is viral, it is most likely to be an enveloped virus (Herbst and others 1996a, b). However, similar fibropapillomas are caused in many vertebrates by papillomaviruses, that is, naked DNA viruses of the family Papovaviridae. Although papillomaviruses were absent from fibropapillomas of green turtles from Florida and Hawaii examined by using electron microscopy, immunohistochemistry and nucleic acid blot probing (Jacobson and others 1989), subsequent development of sensitive polymerase chain reaction (PCR) diagnostics for papillomaviruses has prompted reinvestigation of a possible association between papillomaviruses and sea turtle FP. Lu (1998) used degenerate PCR primers to amplify a DNA fragment which included a short nucleotide sequence motif identical to a sequence in the late structural capsid protein 1 (Li) gene of mammalian papillomaviruses. The fragment was amplified from fibropapillomas, lung, kidney, heart, skin, and cultured cells derived from fibropapillomas, testis and lung of FP-affected green turtles from Hawaii. The data were interpreted to represent detection of papillomaviruses in tumour tissues of green turtles.This short communication reports the results of an assay for papillomaviruses in nucleic acid samples purified from 26 fibropapillomas from 10 green turtles and one loggerhead turtle from Florida. Four pairs of PCR primers with known efficiency of detection were used.The nucleic acid samples used for the PCR templates were obtained by using standard methods of digestion (0.5 g sample plus 50 mg trypsin in 500 VI of 10mM Tris-HCl pH 8, 0-4M sodium chloride, 0-6 per cent sodium dodecyl sulphate [SDS], and 50mM ethylenediaminetetraacetic acid [EDTA], incubated at 37°C until liquified) and phenol:chloroform extraction of 26 cutaneous fibropapillomas from 10 green turtles and one loggerhead turtle stranded along the east coast of Florida (Lackovich and others 1999).The PCR was performed by using a Perkin-Elmer Gene Amp 2400 thermal cycler. Reactions included 10mM Tris-HCl pH 9, 50mM potassium chloride, 0.1 per cent Triton X-100, 2-5 mg template nucleic acid or 500 ng positive control plasmid DNA, 0-2mM deoxynucleoside triphosphates, 50 pmol each primer, and 2-5 U Taq DNA polymerase in 100 1I volumes. For consensus degenerate primer combination MYO9 + MY11, complementa...
