Characterization of Monoclonal Antibodies to California Sea Lion (Zalophus californianus) Immunoglobulin Molecules
IAAAM 2000
Michelle C. Hure1, BS; Donald P. King1, PhD; Brian M. Aldridge1,2, PhD, DACVIM, MRCVS; Frances Gulland2, VetMB, PhD, MRCVS; William Van Bonn3, DVM; Myra Blanchard1, MS; Jeffrey L. Stott1, PhD
1Laboratory for Marine Mammal Immunology, Department of Pathology, Microbiology and Immunology, School of Veterinary Medicine, University of California, Davis, CA, USA; 2The Marine Mammal Center,
GGNRA, Sausalito, CA, USA; 3U.S. Navy Marine Mammal Program, SPAWARSYSCEN, San Diego, CA, USA
Abstract
California sea lions (Zalophus californianus, CSL) are common inhabitants of the Pacific coast
waters and as such comprise a significant proportion of the sick and injured animals treated at rehabilitation centers along
the west coast. In addition, CSLs are excellent sentinels for disturbances in marine and coastal ecosystems, since they feed
high on the marine food web. This species is also recognized as a highly valuable partner to mankind in several open-ocean
work tasks and in performance environments. Unfortunately there is a shortage of reagents and tools that can be used for
health assessment in this species, particularly in comparison to those available for the Pacific harbor seal (Phoca
vitulina).
The aim of this project was to develop immunologic reagents that can be employed in a wide range of
diagnostic and research assays, and thereby enhance our ability to study CSL in health and disease. Since infectious disease
is an important cause of morbidity and mortality in many of the pinniped species treated at rehabilitation centers, we
decided to develop reagents that could be used to study health in captive and free-ranging populations. Monoclonal
antibodies against CSL immunoglobulins (Ig) could be employed to develop a number of diagnostic and research assays. These
assays could have broad application, ranging from population-based epidemiologic studies in large populations, to evaluating
pathogen-specific immune responses in individual animals.
The antigen for producing these monoclonal antibodies was purified CSL serum immunoglobulin. The CSL
immunoglobulin was used to immunize mice and therefore induce the production of anti-CSL Ig producing B cells. Several weeks
after vaccination spleen cells were collected from the mice, and all healthy splenic B cells were immortalized by fusing
them with a commercially available myeloma cell line. To identify and isolate the B cells that produced anti-CSL Ig
antibodies a series of cell expansions and clonings were performed. The cell culture supernatants were evaluated for the
presence of anti-CSL Ig antibodies by sequential analysis in the following assays: 1) ELISA using purified Ig as the antigen
coated onto the plates and 2) ELISA using sera from leptospira seropositive CSLs bound to leptospira proteins. Using this
approach several anti-CSL Ig antibody-producing B cell lines were purified. The specificity of these cell lines is currently
being confirmed by 1) immunoprecipitation of the target antigen for determination of molecular weight and 2) western blot
for identification of subunit (heavy or light chain) specificity and molecular weight of the target antigen. Once these
anti-CSL Ig monoclonal antibodies have been characterized, their utility will be examined by employing them in a number of
serologic assays in both captive and free-ranging populations.