Hydrodynamics-Based Transfer of Human Apolipoprotein A-I Gene to Mice: Study of Factors Affecting the Efficiency and Duration of Gene Expression in the Mouse Liver

Human apolipoprotein A-I gene (apoA-I) inserted into a plasmid expression vector was transferred in vivo into C57Bl/6 mice using hydrodynamic injections into the tail vein. Two types of plasmid expression vectors were used: (1) pCMVcapoAI which contained cDNA of apoA-I driven by the human cytomegalovirus (CMV) early gene promoter and (2) pAlg, which contained a genomic locus of intron-containing apoA-I driven by its own extended 5-regulatory region (APOAI). Hydrodynamic intravenous injections of both expression vectors led to the appearance of human apoA-I mRNA in the liver and human ApoA-I protein in the serum of injected mice. The dynamics of human ApoA-I content in the sera of mice injected with pCMVcapoAI and pAlg were different. When pCMVcapoAI was used, the concentration of human ApoA-I in mouse serum was maximal one day after injection and decreased to zero within the next two weeks. In the case of pAlg, the content of human ApoA-I in serum was maximal (up to 20 g/ml) on days 5–7 after injection and then gradually decreased for several months (six months after injection, for example, it decreased to 25% of the maximal value). Experiments on saved pAlg plasmid isolated from the nuclei of hepatocytes 50 days after injection showed that the plasmid was retained for a long time in the form of an episome. A significant content of human ApoA-I in serum and its long-term persistence after injecting mice with pAlg may be accounted for by the properties of APOAI and/or the exon–intron structure of the apoA-I gene. Injecting mice with different variants of APOAI coupled with the luciferase gene did not lead to long-term expression of luciferase in the liver. It is concluded that the presence of introns in the apoA-I gene is required for its efficient and long-term expression after transfer to mice by means of hydrodynamic injections.     

Effect of TNFα on activities of different promoters of human apolipoprotein A-I gene

Human apolipoprotein A-I (ApoA-I) is a major structural and functional protein component of high-density lipoproteins. The expression of the apolipoprotein A-I gene (apoA-I) in hepatocytes is repressed by pro-inflammatory cytokines such as IL-1β and TNFα. Recently, two novel additional (alternative) promoters for human apoA-I gene have been identified. Nothing is known about the role of alternative promoters in TNFα-mediated downregulation of apoA-I gene. In this article we report for the first time about the different effects of TNFα on two alternative promoters of human apoA-I gene. Stimulation of HepG2 cells by TNFα leads to activation of the distal alternative apoA-I promoter and downregulation of the proximal alternative and the canonical apoA-I promoters. This effect is mediated by weakening of the promoter competition within human apoA-I 5′-regulatory region (apoA-I promoter switching) in the cells treated by TNFα. The MEK1/2-ERK1/2 cascade and nuclear receptors PPARα and LXRs are important for TNFα-mediated apoA-I promoter switching.     

Characterization of Distal and Proximal Alternative Promoters of the Human ApoA-I Gene

Molecular Biology - Human apolipoprotein A-I (ApoA-I) is a major structural and functional protein component of high-density lipoprotein (HDL). ApoA-I constitutes ~75% of the protein content of...     

The functional activity of fractions of coelomocytes of the starfish <Emphasis Type="Italic">Asterias rubens</Emphasis> Linnaeus, 1758

As a result of the centrifugation of the circulating cells of the starfish Asterias rubens in a discontinuous density gradient of sodium diatrizoate, three cell fractions were separated. Small coelomocytes with a high nuclear–cytoplasmic ratio and the lack of granules prevailed in the upper fraction, coelomocytes with small granules evenly distributed in their cytoplasm dominated in the middle fraction, and large coelomocytes with a high content of large granules and vesicles in the perinuclear space were predominant in the bottom fraction. The coelomocytes of the separated fractions were tested for the production of reactive oxygen species, neutral red uptake, capture and internalization of the labeled bacteria Escherichia coli and Staphylococcus aureus, as well as for lytic activity and expression of the ArC3-like gene, which is a homologue of the C3 component of the mammalian complement cascade. Cells of the upper fraction manifested the most pronounced ability for the expression of the C3 gene homologue in response to stimulation with bacterial lipopolysaccharide. Coelomocytes of the middle fraction were distinguished by a pronounced ability to produce reactive oxygen species and phagocytosis, whereas the cells of the lower fraction had a high level of hemolytic activity and neutral red uptake.