Direct injection of indicators for calcium imaging at the Drosophila larval neuromuscular junction.

Calcium imaging is a technique in which Ca(2+)-binding molecules are loaded into live cells and as they bind Ca(2+) they "indicate" the concentration of free calcium through a change in either the intensity or the wavelength of light emitted (fluorescence or bioluminescence). There are several possible methods for loading synthetic Ca(2+) indicators into subcellular compartments, including topical application of membrane-permeant Ca(2+) indicators, forward-filling of dextran conjugates, and direct injection. Calcium imaging is a highly informative technique in neurobiology because Ca(2+) is involved in many neuronal signaling pathways and serves as the trigger for neurotransmitter release. This article describes the direct injection of Ca(2+) indicators at the Drosophila larval neuromuscular junction (NMJ). This technique allows rapid loading of most Ca(2+) indicators, but there are drawbacks in that it is a difficult technique to master and requires additional electrophysiological equipment. Also, Ca(2+) indicators that are easily injected are usually susceptible to compartmentalization.