Dependences of intracellular calcium signals on the concentrations of endogenous buffers (slow, parvalbumin, and fast, calmodulin) and a calcium-sensitive fluorophore (Fura-4F) were investigated on mathematical models of compartments of the reconstructed dendrite of a cerebellum Purkinje neuron. A Ca2+-storing cistern of the endoplasmic reticulum (ER) was present in the dendrite. Calcium signals developed when the neuron generated responses to single synaptic excitation or intrinsic non-periodical impulse activity. The dynamics of the buffer binding capacity were also studied; this capacity was characterized by the ratio of concentrations of bound and free calcium or concentration increments of the latter. The plasma membrane of the dendrite possessed ion channels (including those of synaptic currents) and the calcium pump characteristic of the mentioned neuron. Model equations took into account Ca2+ exchange between the cytosol, buffers, ER, and extracellular medium, as well as diffusion processes. The ER membrane contained the calcium pump, leakage channels, and channels of calcium-induced release and inositol-3-phosphate-dependent releases of Ca2+. The ER cistern occupied 1 to 36% of the intracellular volume. Upon different occupancies of the dendrite by the organelle store, an increase in the concentration of the slow buffer insignificantly decreased the cytosolic Ca2+ transients with no effect on their shape. The fast buffer and the dye with similar kinetic properties caused slowing down of the rising phase of Ca2+ transients, decrease in the early component, and increase in the late component of the latter. In the case of nonperiodical and asynchronous intrinsic oscillations of the membrane potential typical of asymmetrical active dendrites, the slow buffer, like the ER store, bound more Ca2+ in compartments of compatible sizes and fillings by the organelles belonging to those metrically asymmetrical branches, which, on average, stayed longer in the state of high depolarization; this provided a greater Ca2+ entry from outside. Hence, the pattern of structural/functional organization of calcium signalization in the dendrites can be complemented in the part of both the direct influences of local microgeometry of the dendrite and the indirect ones related to global macrogeometry of the dendritic arborization.