Immunological assays of hemocytes in the Northern Quahog Mercenaria mercenaria

Yangqing Zeng; Yuanzi Huo; Huiping Yang

doi:10.1016/j.fsi.2021.09.006

Immunological assays of hemocytes in the Northern Quahog Mercenaria mercenaria

Fish Shellfish Immunol. 2021 Nov:118:261-269. doi: 10.1016/j.fsi.2021.09.006. Epub 2021 Sep 8.

Authors

Yangqing Zeng¹, Yuanzi Huo¹, Huiping Yang²

Affiliations

¹ School of Forest, Fisheries, and Geomatics Sciences, Institute of Food and Agricultural Sciences, University of Florida, 7922 NW 71st Street, Gainesville, FL, 32653, USA.
² School of Forest, Fisheries, and Geomatics Sciences, Institute of Food and Agricultural Sciences, University of Florida, 7922 NW 71st Street, Gainesville, FL, 32653, USA. Electronic address: huipingyang@ufl.edu.

PMID: 34506884
DOI: 10.1016/j.fsi.2021.09.006

Abstract

The northern quahog Mercenaria mercenaria (commonly named hard clam) is an important aquaculture and fishery species along the Atlantic west coast. Environmental stresses, such as heat shock, fluctuating salinity, and harmful algal blooms are major challenges for clam aquaculture. In response to environmental stresses, hemocytes would change dynamically for defense and immunity. The goal of this study was to characterize basic immunological assays of hemocytes in the northern quahog by use of flow cytometry. The objectives were to: 1) develop a non-lethal method for hemolymph collection and dilution; 2) verify the capability of flow cytometry for hemocyte count and type identification through comparison with microscopic observation; 3) validate hemocyte viability assay based on plasma membrane integrity, and 4) develop hemocyte phagocytosis assay by use of fluorescein labeled microbeads. A non-lethal hemocyte collection method was developed using needle insertion through the ligament. Osmolality measurement of serum was the same as that of culture seawater. The pH measurement of serum (7.2) was significantly different from that of culture seawater (8.4). By microscopic observation, three types of hemocytes were identified with granulocytes, the dominant cell type (70 ± 16%), agranulocyte (14 ± 4%), and blast-like cell (16 ± 4%), and no differences were found from the measurements by flow cytometer on FSC/SSC plot (cell size/granularity). The viability of hemocytes based on plasma membrane integrity was 88 ± 6% ranging from 70 to 97% (n = 60, three populations), and viability protocol was further validated with the pre-set expected viability (p ≥ 0.424). Phagocytosis assay of hemocytes with fluorescence beads showed a mean capacity of 10 ± 5% (n = 60, three populations). Incubation time (up to 6 h) or bead concentrations (2:1 or 5:1 to hemocytes) did not affect the phagocytosis measurement. Overall, this study reported the basic characteristics of hemolymph (serum and hemocytes) of northern quahogs. It is expected that the assay methodologies will be applied to evaluation of hemocyte responses to environmental stresses for clam aquaculture.

Keywords: Agranulocyte; Blast-like cell; Flow cytometry; Granulocyte; Hemocyte; Mercenaria mercenaria; Non-lethal sampling; Northern quahogs; Phagocytosis; Viability.

MeSH terms

Animals
Aquaculture
Hemocytes / immunology*
Hemolymph / immunology
Mercenaria / immunology*
Phagocytosis
Seawater