Immune activation upregulates lysozyme gene expression in Aedesaegypti mosquito cell culture
Article first published online: 7 JUL 2008
DOI: 10.1046/j.1365-2583.2000.00216.x
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How to Cite
Gao, Y. and Fallon, A. M. (2000), Immune activation upregulates lysozyme gene expression in Aedesaegypti mosquito cell culture. Insect Molecular Biology, 9: 553–558. doi: 10.1046/j.1365-2583.2000.00216.x
Publication History
- Issue published online: 7 JUL 2008
- Article first published online: 7 JUL 2008
- Received 4 May 2000;accepted 10 July 2000.
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Keywords:
- insect immunity;
- insect cell lines;
- immunity proteins;
- RT-PCR;
- Northern blot;
- Southern blot
Abstract
After stimulation with heat-killed bacteria, cultured cells from the mosquito Aedesaegypti (Aag-2 cells) secreted an induced protein with a mass of ≈ 16 kDa that cross-reacted with antibody to chicken egg lysozyme. To investigate whether lysozyme messenger RNA is induced in bacteria-treated cells, we used polymerase chain reaction-based approaches to obtain the complete lysozyme cDNA from Aag-2 cells. The deduced protein contained 148 amino acids, including a 23 amino acid signal sequence. The calculated mass of the precursor protein is 16 965 Da, which is processed to yield a mature lysozyme of 14 471 Da with a calculated pI of 10.1. The lysozyme from Ae. aegypti shared 50% amino acid identity with lysozymes from Anophelesgambiae and Anophelesdarlingi, which in turn shared 70% identity between each other. Northern analysis with the lysozyme cDNA probe showed induction of a 1.3 kb messenger RNA during the first 3 h after treatment of Aag-2 cells with heat-killed bacteria, followed by maximal expression 12–36 h after treatment. Southern analysis suggested that the gene likely occurs as a single copy in the genome of Aag-2 cells.

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