Fig. 1

Comparison of wt and grk follicles. a The dorsal side of wt S10B is defined by a thicker, columnar follicular epithelium (FE) and by an anterodorsal position of the oocyte nucleus (ON, red circle; cFC, centripetal follicle cells; mFC, mainbody follicle cells; pFC, posterior follicle cells). bgrk S10B lacks dorsoventral (d-v) polarity and is characterised by a uniform cuboidal, ventralised FE covering the oocyte (Ooc). While, in wt S10B, border cells (BC) are located close to the ON, in grk S10B, disrupted body-axis formation leads to undefined positioning of BC amongst the nurse cells (NC). The grk ON is often located at the posterior end of the Ooc in a typical protrusion. c Transheterozygous combinations of grk alleles HF48 and 2B6 result in ventralised grk follicles of all vitellogenic stages (S8–14; bright-field image). In S12–14, wt-typical dorsal respiratory appendages are missing and a second micropylar structure appears at the posterior end. d To visualise basal microfilaments (bMF) and microtubules (MT) in the FE, tangential optical sections using structured-illumination microscopy (SIM; focal plane: red line) were used. For analysis of V_mem- and pH_i-patterns, median optical sections (SIM; focal plane: turquoise line) were used. e Quantification of transversal (e₁) and anteroposterior (a-p; e₂) gradients of V_mem and pH_i, respectively, in the FE of S10B. Example of a grk follicle (SIM) where DiBAC-fluorescence intensities of FE₁ (area marked in yellow) and FE₂ (white) as well as of aFE (red) and pFE (blue) were measured using ImageJ (“mean grey value”). In wt follicles, the d-v axis was identified via the anterodorsal position of the ON, and the fluorescence intensities of the dorsal and ventral FE were quantified accordingly