Abalone herpesvirus (AbHV) infection of cultured abalone Haliotis diversicolor supertexta has induced high mortality rates in Taiwan in 2003. The histopathologic study has revealed AbHV is prone to infect neurotic tissues and has caused ganglioneuritis in moribund abalone. The purpose of this study is to express the outer membrane recombinant protein fragment ORF44 of AbHV and use this protein as an antigen to prepare the polyclone antibody, then apply in the immunohistochemistry study as diagnostic tool. We have designed a specific primers and amplified this ORF44 fragment by PCR. The amplifed DNA fragment was cleaved by restriction enzymes and inserted into pET24a (+) vector. The ORF44 expression plasmid was transformed into E. coli （BL21（DE3）） to construct the recombinant ORF44 protein with 110 amino acid residues. The IPTG-induced soluble recombinant protein was purified by a nickel-nitrilotriacetic acid (Ni2+_NTA) agarose metal ion column affinity chromatography via 6X-histidines on its C-terminal. By SDS-PAGE analysis, the molecular mass of the purified recombinant protein was about 13 kDa. The polyclonal anti-ORF44 antiserum was prepared from rabbit immunized with the adjuvant-emulsified recombinant ORF44 protein. By using the Western blotting hybridization and immunohistochemistry, the antiserum was proved to recognize the abalone hepesvirus ORF44 proteins and the neurologic lesion of AbHV-infected abalone.