Pathways of inositol pyrophosphate metabolism in S. cerevisiae.

Cytosolic concentrations of 5-IP7, 1-IP7 and IP8.

(A) Inositol pyrophosphate concentrations in the cytosol. The indicated strains were grown logarithmically in SC medium containing 7.5 mM of Pi (30°C, 150 rpm, overnight). When OD600nm reached 1 (1 x 107 cells/ml), 1 ml of culture was extracted with perchloric acid and analyzed for PP-IPs by CE-ESI-MS. The y-axis provides the estimated cytosolic concentrations based on an average cell volume of 42 fL. Means (n=4) and standard deviations are indicated.

(B) Evolution of Inositol pyrophosphate species during Pi starvation. Cells were grown as in A, washed twice with Pi starvation medium and further incubated in Pi starvation medium. The inoculum for the samples bound to be extracted after different times of further incubation in starvation medium was adjusted such that all samples had similar OD600nm at the time of harvesting (OD600nm=0.5 for 30 min and 60 min samples; OD600nm=0.4 for 120 min and 240 min samples; OD600nm=0.25 for 360 min samples). At the indicated times in starvation media, 1 ml aliquots were extracted analyzed for PP-IPs as in A. The data was normalized by the number of cells harvested before calculating cytosolic concentrations. Means and standard deviations are given (n=3).

(C) Depletion of 5-IP7 in starving vip1Δ cells. The indicated cells were grown in Pi-replete medium and then transferred to Pi starvation medium as in B. At the indicated times, samples were extracted and analyzed for 5-IP7 as in A. Means and standard deviations (n=4) are shown as solid lines and shaded areas, respectively.

Inhibition of the PHO pathway by excessive 5-IP7.

The indicated cells expressing Pho4yEGFP and the histone Hta2mCherry as a nuclear marker were logarithmically grown in Pi-replete SC medium, washed, and transferred to Pi starvation medium as in Fig. 2A.

(A) Subcellular localization of Pho4yEGFP was analyzed on a spinning disc microscope. Cells are shown in the presence of 7.5 mM of Pi (+ Pi) or 30 min after the shift to Pi starvation (−Pi) medium. Yellow lines surrounding the cells illustrate the segmentation performed by the algorithm that was used to quantify Pho4yEGFP distribution in B. Scale bar: 5 μM. λex: 470 nm; λem: 495-560 nm.

(B) Average intensity of Pho4yEGFP fluorescence was determined by automated image segmentation and analysis. Pho4yEGFP localization is quantified by the ratio of the average fluorescence intensities in the nucleus over the average fluorescence intensity in the cytosol (IN/IC). XXX cells were analyzed per condition and experiment. n=3. Means and standard deviation are indicated.

(C) Activation of the PHO5 promotor. Cells expressing the prPho5-yEGFP reporter construct from a centromeric plasmid were grown in Pi-replete medium (7.5 mM Pi) as in Fig. 2A, and then shifted to Pi starvation medium or kept in Pi replete medium. After 4 h of further incubation, fluorescence intensity of the same number of cells was measured in a Spectramax EM microplate reader. λex: 480 nm; λem: 510 nm. n=3. Means and standard deviation are indicated. *Activation of the Pho84 promotor. Cells expressing the prPho5-yEGFP reporter construct from a centromeric plasmid were treated and analyzed as in C. *** p<0.0001; *** p<0.001; ** p<0.01; n.s.: not significant

Effect of Vip1, Kcs1 and Pho81 on the time course of Pho4 translocation and PHO-gene activation.

The indicated cells were logarithmically grown in Pi-replete SC medium, washed, and transferred to Pi starvation medium as in Fig. 2A. At the indicated times after transfer to Pi-starvation medium, they were analyzed for Pho4 localization, prPHO5-yEGFP expression, or prPHO84-yEGFP expression, using assays as in Fig. 3.

(A) Cells expressing Pho4yEGFP and the histone Hta2mCherry as a nuclear marker, shown in the presence of 7.5 mM of Pi (+ Pi) or after 90 min of Pi starvation (−Pi). Pictures were taken on a widefield fluorescence microscope equipped with a stage-top incubator (kept at 30°C) and an IBIDI flow chamber. Only the GFP-channel is shown. Scale bar = 5 μM. λex: 470 nm; λem: 495-560 nm.

(B) Distribution of Pho4yEGFP between the nucleus and cytosol was quantified in the cells from A at various timepoints of Pi starvation. 100-200 cells were analyzed per condition and experiment at each timepoint. The solid lines and the shaded areas indicate the means and standard deviation, respectively.

(C) Activation of the PHO5 promotor. Cells expressing the prPho5-yEGFP reporter construct from a centromeric plasmid were grown in Pi-replete medium, shifted to Pi starvation medium, and analyzed for GFP fluorescence intensity (as in Fig. 3C) at the indicated timepoints of starvation. λex: 480 nm; λem: 510 nm. n=3. The solid lines and the shaded areas indicate the means and standard deviation, respectively.

(D) Activation of the PHO84 promotor. As in C, but with cells expressing prPHO84-yEGFP as reporter.

SPX-dependent activation of the PHO pathway.

Cells were logarithmically grown in Pi-replete SC medium as in Fig. 2A, washed, and incubated for further 4 h in medium with 7.5 mM of Pi (+ Pi), or in starvation medium (−Pi).

(A) Pho4 relocation. The indicated cells expressed Pho4yEGFP from its genomic locus. At the end of the 4 h starvation period, GFP fluorescence was imaged on a spinning disc microscope. Scale bar: 5 µm. λex: 488 nm; λem: 500-530 nm.

(B) Quantification of the nuclear localization of Pho4yEGFP. Images from A were subjected to automated segmentation and quantification of the average fluorescence intensity in the nucleus and cytosol as in Fig. 3B. 100-200 cells were quantified per sample. n=3 experiments.

(C) Pho81yEGFP localization and expression. The cells expressed the indicated variants of Pho81yEGFP from its genomic locus. At the end of the 4 h growth period, GFP fluorescence was imaged as in A.

(D) Quantification of the total cellular fluorescence of Pho81yEGFP. Images from C were subjected to automated segmentation and the average fluorescence intensity of the entire cells was quantified as in Fig. 3B. 100-200 cells were quantified per sample. n=3 experiments.

(E) Pho81yEGFP expression assayed by blotting. Whole-cell protein extracts were prepared from cells expressing the indicated variants of Pho81yEGFP, which had been grown in Pi-replete SC medium as in Fig. 2A. Proteins were analyzed by SDS-PAGE and Western blotting of Pho81yEGFP. Vps1 was decorated as a loading control.

(F) Quantification of Pho81yEGFP blotting. Bands from experiments as in E were quantified on a LICOR Odyssey infrared fluorescence imager. The signals from wildtype cells were set to 1. Means and standard deviations are shown. n=3. **** p<0.0001; *** p<0.001; ** p<0.01; * p<0.05.

Localization of Pho81yEGFP in pho80R121K and pho80E154V loss-of-affinity mutants.

Cells were logarithmically grown in Pi-replete SC medium as in Fig. 2A, washed, and incubated for further 4 h in medium with 7.5 mM of Pi (+ Pi), or in starvation medium (−Pi).

(A) Pho81 imaging. Cells expressing Pho81yEGFP and the indicated variants of Pho80 from their genomic loci were imaged on a spinning disc microscope after 4h of growth in the presence of 7.5 mM Pi (+ Pi), or after 4h of Pi starvation (−Pi). Scale bar = 5 μM. λex: 488 nm; λem: 500-530 nm. Note that the fluorescent dots visible in pho81Δspxcells are not nuclei because they are too small and at positions where nuclei are not found. Their location was not further investigated because it is not essential for this study.

(B) Quantification of the nuclear localization of Pho81yEGFPin pho80R121K cells. Images from A were subjected to automated segmentation and quantification of the average fluorescence intensity in the nucleus and cytosol as in Fig. 3B. 100-200 cells were quantified per sample. n=3 experiments.

(C) Quantification of the nuclear localization of Pho81yEGFP in pho80E154V mutants was performed as in B.

Structure predictions of the minimum domain in complex with Pho80

Alphafold multimer was used to generate the following structure predictions:

(A) Pho80 in complex with the minimum domain of Pho81 (aa 645-724).

(B) Pho80 in complex with Pho81.

Coloring: Beige - Pho80; red - E154, R121 of Pho80; blue: Pho81 minimum domain; green - central region of the Pho81 minimum domain that is critical for Pho85/Pho80 inhibition (aa 690-701); yellow: SPX domain of Pho81; grey - rest of Pho81 without assigned function.

Pho81 residues leading to constitutive activation of the PHO pathway

The image shows an Alphafold prediction of the Pho81 SPX domain (aa 1-215) in yellow. Basic residues of the PP-IP binding site have been identified by structure matching with the IP6-associated SPX domain of VTC4 from Chaetomium thermophilum (PDB 5IJP). They are labeled in red. Residues from random mutagenesis screens, which lead to constitutive activation of the PHO pathway are labeled in green.

Working model on the control of the PHO pathway through 1,5-IP8 and Pho81.

At high Pi concentrations, inositol pyrophosphates accumulate. 1,5-IP8 preferentially binds the SPX domain of Pho81, which labilizes the interaction of Pho81 with Pho80 and prevents Pho81 from inhibiting Pho85/Pho80 kinase.

Determination of cell dimensions from trypan blue stained wild-type cells.

Segmentation of fluorescence microscopy time-lapse experiments.

The subcellular localization of Pho4-yoEGFP has been quantified from time-lapse fluorescence microscopy experiments. This quantification required the segmentation of microscopy images to discriminate cytosolic and nuclear compartments. To this end, the hta2 histone of Pho4-yoEGFP strains has been tagged with mCherry. Nuclei were segmented using mCherry fluorescence images while the cell contours were segmented using brightfield images. Cell segmentation and the fluorescence quantification were performed using the General Analysis 3 module of the NIS Elements software (Nikon). (A) The brightfield and two fluorescence images of the same field are shown. Yellow lines indicate the boundaries of the cells and nuclei that have been recognized by the algorithm. (B) Flow chart of the commands of the NIS Elements General Analysis 3 suite used for the segmentation. The script has been deposited and can be downloaded from ******.

Myo-inositol polyphosphate binding pocket of yeast SPX domains.

(A) Crystal structure close-up view of C. thermophilum Vtc4 SPX domain complexing IP6 (5IJP). (B) Structure prediction (generated with SWISS-MODEL) of the S. cerevisiae Pho81 SPX domain revealing the potential conserved PBC and KSC clusters. (C) Alignment of the conserved residues myo-inositol polyphosphate binding motifs of Pho81 and of the different VTC subunits.

Loss of PP-IPs from siw14Δ cells upon Pi starvation.

The indicated strains were grown logarithmically in SC medium containing 7.5 mM of Pi (30°C, 150 rpm, overnight). The cells were spun down, washed twice with Pi starvation medium and further incubated in Pi starvation medium or in SC with Pi for 2h. The inoculum for the samples for this final 2h incubation was adjusted such that all samples had an OD600nm of 1 (107 cells/ml) at the time of harvesting. After the two hours incubation, 1 ml of culture was extracted with perchloric acid and analyzed for PP-IPs by CE-ESI-MS. The data was normalized by the number of cells harvested before calculating cytosolic concentrations. The y-axis provides the estimated cytosolic concentrations based on an average cell volume of 42 fL. Means (n=4) and standard deviations are indicated.

Inositol pyrophosphate analysis in C. neoformans

Cells were logarithmically grown in synthetic complete (SC) medium for 17h up to an OD600nm of 1. Cells were sedimented by centrifugation, resuspended in SC without Pi, and incubated further. At the indicated times, aliquots were extracted with perchloric acid. PP-IPs were enriched on TiO2 beads and analyzed by CE-MS. Concentrations of 1,5-IP8, 5-IP7 and 1-IP7 in the extracts were determined by comparison with added synthetic 13C-labeled PP-IP standards. The graphs provide the concentrations in the extracts. n=4; means and standard deviations are indicated. The IPP analysis data were normalized to the OD600 of the culture at the given time point.

Strains used in this study

Plasmids used in this study

Oligonucleotides used in this study

Parameters for MRM transitions