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Nanyang Technological University

Inducing Neuroinflammation in Zebrafish Larvae with a Lipopolysaccharide Injection

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Take anesthetized zebrafish larvae in a dish lined with agarose gel and ensure that the brain faces upward for injection.

Position the dish under a microscope to visualize the brain ventricles, which are fluid-filled cavities within the developing brain.

Take a microinjection needle containing a solution of lipopolysaccharides, or LPS, a bacterial component to trigger an immune response.

Position the needle above the brain tectum, a region containing neurons and resident immune cells, particularly microglia.

Puncture the brain with the needle and inject the LPS solution into the ventricle.

Microglia in the surrounding tissue binds to LPS through toll-like receptors.

The binding triggers the release of pro-inflammatory cytokines, which recruit neutrophils to the site, leading to neuroinflammation.

Neutrophils generate bursts of reactive oxygen species and release proteolytic enzymes, resulting in neuronal death.

Transfer the neuroinflammation-induced larvae into a culture medium to maintain them for downstream assays.

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Inducing Neuroinflammation in Zebrafish Larvae with a Lipopolysaccharide Injection

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