Developmental Biology

Repetitive increases of intracellular calcium ions (Ca²⁺ oscillations) control cellular functions in various biological events, including meiotic resumption after fertilization. Sperm-derived substances enter the cytoplasm of mature oocytes by sperm fusion, causing Ca²⁺ oscillations. Sperm-independent Ca²⁺ oscillations are also induced in immature oocytes isolated from the ovaries of neonatal to adult mice. The presence of Ca²⁺ oscillations may contribute to subsequent oocyte quality; however, its physiological role and molecular mechanism are unclear. Here, we describe a method of collecting immature oocytes from the ovaries of juvenile (12, 15, and 21 days after birth) and adult mice and monitoring their Ca²⁺ oscillations. Since mouse oocytes are larger than other types of cells, they are a useful model for studying spatiotemporal patterns and the mechanism of Ca²⁺ oscillations in various types of cells. This method can be applied to other rodents due to similarities in oocyte size and developmental processes. Furthermore, the use of various fluorescent probes enables visualization of organelle rearrangement. The mechanism of interaction between oocytes and somatic cells differs between juvenile and adult mice. Therefore, two distinct methods are employed for oocyte collection.

Calcium signalling in the endocardium is critical for heart valve development. Calcium ion pulses in the endocardium are generated in response to mechanical forces due to blood flow and can be visualised in the beating zebrafish heart using a genetically encoded calcium indicator such as GCaMP7a. Analysing these pulses is challenging because of the rapid movement of the heart during heartbeat. This protocol outlines an imaging analysis method used to phase-match the cardiac cycle in single z-slice movies of the beating heart, allowing easy measurement of the calcium signal.

Visualizing the function of pancreatic β-cells in vivo has been a long-sought goal for β-cell researchers. Unlike imaging of β-cells in mammalian species with conventional positron emission tomography and single-photon emission computed tomography, which only provides limited spatial-temporal resolution, transparent zebrafish embryos are a unique model that allows high-resolution fluorescent imaging of β-cells in their native physiological microenvironment in vivo. Here, we detail a protocol for real-time visualization of individual β-cell function in vivo in a non-invasive manner, through combination of a novel transgenic zebrafish reporter line Tg (ins:Rcamp1.07) with both a commercial spinning-disc confocal microscope and an in-house developed super-resolution microscope (2P3A-DSLM). The protocol described here allows for the longitudinal monitoring of dynamic calcium activities from heterogeneous β-cells in early developing zebrafish embryos and is readily adaptable for use in imaging other important processes in islet biology, as well as screening new compounds that can promote β-cell function or maturation using a living whole organism system.

Extracellular ATP is a potent signaling molecule that stimulates intracellular calcium responses through purinergic (P2) receptors in mammalian cells. While extracellular ATP and intracellular calcium can be measured separately, simultaneous monitoring can offer additional insights into P2 receptor physiology. This protocol takes advantage of the overlapping fluorescence spectra between the ATP-detection substrate luciferin and calcium indicator dye Fura2. Mammalian cells are loaded with Fura2-AM and live-cell recordings are acquired in the presence of a luciferin-luciferase imaging solution. This protocol allows to study stimulus-induced ATP release and directly relate changes in extracellular ATP concentration to observed calcium responses.