Пример #1
0
def main():

    basedir = os.path.join(this_dir, "../../datasets/LSM700_63x_sigb")

    if not USE_CACHE_PLOTS:
        cell_df = pd.read_hdf(os.path.join(basedir, "single_cell_data.h5"),
                              "cells")
        file_df = filedb.get_filedb(os.path.join(basedir, "file_list.tsv"))
    else:
        file_df = None
        cell_df = None

    time = 48
    location = "center"
    slice_srt, slice_end = 5, 7  #10, 15
    #slice_srt, slice_end = 5, 6 #10, 15 #
    # There is no major difference between 5-6 and 7-8, just the QP skew is bigger in 5-6
    #slice_srt, slice_end = 7, 8 #10, 15
    # Moving to 2um because it makes the plots look nicer.

    # fig, ax = plt.subplots(4, 2)
    # axhisto = ax[:, 1]
    # aximage = ax[:, 0]
    fig, ax = plt.subplots(2, 4)
    axhisto = ax[1, :]
    aximage = ax[0, :]

    for i, (name, path, roi, chans) in enumerate(image_list):
        impath = os.path.join(image_base_dir, path)
        aximage[i] = subfig_draw_bin.get_figure(aximage[i],
                                                name,
                                                impath,
                                                roi,
                                                chans,
                                                FP_max_min,
                                                (slice_srt, slice_end),
                                                add_scale_bar=i == 0)
        aximage[i].set_title("")
        aximage[i].text(imgletter_lab[0],
                        imgletter_lab[1],
                        topletters[i],
                        transform=aximage[i].transAxes,
                        **letter_settings,
                        color="white")

    text_x = 0.40
    text_top = 0.85
    line_sep = 0.15
    title_loc, cv_loc, samp_loc, cell_loc = [
        (text_x, text_top - (line_sep * i)) for i in range(4)
    ]

    strain_map, des_strain_map = strainmap.load()
    gchan = "green_raw_bg_meannorm"
    rchan = "red_raw_bg_meannorm"
    if not USE_CACHE_PLOTS:
        cell_df = cell_df[cell_df[rchan] > 0].copy()

    #max_val = 30000
    #max_val = 1.0 #6.0 #20000
    #gmax_val = 1.0 #7.5
    max_val = 6.5  #2.5
    gmax_val = 6.5  #0.75
    nbins = 150
    rbins = (0, max_val, nbins)
    gbins = (0, gmax_val, nbins)
    percentile = 0  #99
    list_of_histos = [("wt_sigar_sigby", rchan, "WT P$_{sigA}$-RFP",
                       figure_util.strain_color["JLB021"]),
                      ("wt_sigar_sigby", gchan, "WT P$_{sigB}$-YFP",
                       figure_util.strain_color["JLB021"]),
                      ("delqp_sigar_sigby", gchan, "ΔrsbQP P$_{sigB}$-YFP",
                       figure_util.strain_color["JLB039"]),
                      ("delru_sigar_sigby", gchan, "ΔrsbRU P$_{sigB}$-YFP",
                       figure_util.strain_color["JLB088"])]
    print("-----------")
    for i, (strain, chan, label, color) in enumerate(list_of_histos):
        print(label)
        strain_df = None
        if not USE_CACHE_PLOTS:
            fids = file_df[(file_df["time"] == time)
                           & (file_df["location"] == location) &
                           (file_df["strain"] == des_strain_map[strain])].index
            strain_df = cell_df[cell_df["global_file_id"].isin(fids)]

        dset = time, location, strain
        plot_args = {"color": color, "max_min": "std", "mode_mean": False}
        tbins = gbins
        if "red" in chan:
            tbins = rbins

        args = (axhisto[i], strain_df, chan, tbins, (slice_srt, slice_end),
                dset, percentile, USE_CACHE_PLOTS, this_dir, plot_args)
        axhisto[i], _, meandmed = subfig_indivfile_histo.get_figure(*args)
        axhisto[i].text(1.0,
                        hisletter_lab[1],
                        label,
                        horizontalalignment='right',
                        verticalalignment='top',
                        color="black",
                        fontsize=plt.rcParams["axes.titlesize"],
                        transform=axhisto[i].transAxes)

        axhisto[i].text(hisletter_lab[0],
                        hisletter_lab[1],
                        letters[i],
                        transform=axhisto[i].transAxes,
                        **letter_settings)

    #leg = axhisto[0].legend(loc="center right")

    #axhisto[-1].set_xlabel("Mean normalised cell fluorecence")
    axhisto[0].set_ylabel("Percentage of cells")

    axhisto[0].set_xlim(0, max_val)
    for a in np.ravel(axhisto):
        #a.set_ylabel("Percentage of cells")
        a.set_xlabel("Mean normalised cell fluorecence")
        a.set_ylim(0, 5)
        a.set_xlim(0, gmax_val)
        a.tick_params(axis='x', which='both',
                      direction='out')  #, length=2, pad=0)
        a.tick_params(axis='y', which='both',
                      direction='out')  #, length=2, pad=0)

    # for a in axhisto[:-1]:
    #     a.set_xticklabels([])
    for a in axhisto[1:]:
        a.set_yticklabels([])

    filename = "demo_longtail"
    #fig.subplots_adjust(left=000, ri0ht=0.98, top = 1.0, bottom=0.06, hspace=0.08, wspace=0.2)
    #width, height = figure_util.get_figsize(figure_util.fig_width_small_pt, wf=1.0, hf=1.7)
    fig.subplots_adjust(left=0.05,
                        right=0.99,
                        top=1.0,
                        bottom=0.10,
                        hspace=0.08,
                        wspace=0.15)
    width, height = figure_util.get_figsize(figure_util.fig_width_big_pt,
                                            wf=1.0,
                                            hf=0.5)
    fig.set_size_inches(width, height)
    figure_util.save_figures(fig, filename, ["png", "pdf"], this_dir)
#         "cr_max":10000,
#         "cg_min":2000,
#         "cg_max":(2**14), }]
# height = 260 * 20
# width = 700 * 20
# i = files[0]
# spimg_ax = subfig_spore_image.plot_big_image(spimg_ax,
#                                         sp_image_basedir + i["Path"],
#                                         this_dir, # cache path.
#                                         ((i["y"], i["y"] + height),
#                                         (i["x"], i["x"] + width)),
#                                         (height, width),
#                                         i, vertical=False, scalebar=True)
# letter_lab = (-0.10, 0.98)
# for l, a in zip(figure_util.letters, [spimg_ax, spcount_ax, cellcount_ax]):
#     a.text(letter_lab[0], letter_lab[1], l, transform=a.transAxes, fontsize=figure_util.letter_font_size)

filename = "spore_grad_density_compare"
width, height = figure_util.get_figsize(figure_util.fig_width_small_pt,
                                        wf=1.0,
                                        hf=1.1)
fig.subplots_adjust(left=0.1, right=0.95, top=0.98, bottom=0.09,
                    hspace=0.35)  #, wspace=0.25)

fig.set_size_inches(width, height)
figure_util.save_figures(fig, filename, ["pdf", "png"],
                         os.path.dirname(__file__))
# print("request size : ", figure_util.inch2cm((width, height)))
# fig.savefig(filename + ".png", dpi=dpi)
# fig.savefig(filename + ".pdf", dpi=dpi)
# figure_util.print_pdf_size(filename + ".pdf")
Пример #3
0
letter_settings = {
    "horizontalalignment": "center",
    "verticalalignment": "top",
    "fontsize": figure_util.letter_font_size,
    "color": "black",
}

x1 = 0.02
aximg.text(x1, 0.995, "B", transform=figall.transFigure, **letter_settings)
aximg.text(x1, 0.64, "C", transform=figall.transFigure, **letter_settings)
aximg.text(x1, 0.50, "D", transform=figall.transFigure, **letter_settings)
aximg.text(x1, 0.36, "E", transform=figall.transFigure, **letter_settings)
aximg.text(x1, 0.22, "F", transform=figall.transFigure, **letter_settings)

x2 = 0.53
aximg.text(x2, 0.64, "G", transform=figall.transFigure, **letter_settings)
aximg.text(x2, 0.50, "H", transform=figall.transFigure, **letter_settings)
aximg.text(x2, 0.36, "I", transform=figall.transFigure, **letter_settings)
aximg.text(x2, 0.22, "J", transform=figall.transFigure, **letter_settings)

filename = "pad_movie_tracemain"

width, height = figure_util.get_figsize(figure_util.fig_width_small_pt,
                                        wf=1.0,
                                        hf=1.0)
figall.set_size_inches(width, height)
figall.subplots_adjust(left=0.15, right=0.99, top=1.0, bottom=0.1)
# hspace=0.05)
print("request size : ", figure_util.inch2cm((width, height)))
figure_util.save_figures(figall, filename, ["png", "pdf"], this_dir)
Пример #4
0
##################
im = skimage.io.imread(os.path.join(this_dir, "delru_bf10_col2_strip.png"))
ax_fstrip.imshow(im, interpolation="bicubic")
ax_fstrip.grid(False)
ax_fstrip.axis("off")

axes = [ax_exprmt, ax_gradnt, ax_fstrip, ax_pulses]
letter_style = {
    "verticalalignment": "top",
    "horizontalalignment": "right",
    "fontsize": figure_util.letter_font_size,
    # "color": "red"
}

letter_x = 0.03
axes[0].text(letter_x, 0.995, "A", transform=fig.transFigure, **letter_style)
axes[1].text(0.47, 0.995, "B", transform=fig.transFigure, **letter_style)
axes[2].text(letter_x, 0.63, "C", transform=fig.transFigure, **letter_style)
axes[3].text(letter_x, 0.26, "D", transform=fig.transFigure, **letter_style)

filename = "bf_movie_main"
# width, height = figure_util.get_figsize(figure_util.fig_width_big_pt, wf=1.0, hf=0.5 )
width, height = figure_util.get_figsize(figure_util.fig_width_small_pt,
                                        wf=1.0,
                                        hf=1.3)
fig.subplots_adjust(left=0.095, right=0.97, top=0.97,
                    bottom=0.06)  # , hspace=0.25, wspace=0.25)

fig.set_size_inches(width, height)  # common.cm2inch(width, height))
figure_util.save_figures(fig, filename, ["png", "pdf"], base_dir=this_dir)
Пример #5
0
def main():
    curve_score_methods = {
        "std":
        ("Standard deviation", (0.0, 1.0), lambda d, h, b: np.std(d)),  # 1.5,
        "mean": ("Mean", (0.0, 4.0), lambda d, h, b: np.mean(d)),
        "cv": (
            "Coefficient of variation",
            (0.3, 0.8),
            lambda d, h, b: scipy.stats.variation(d),
        ),
        # "skew": ("modern skew",
        #        0.0, 3.0,
        #        lambda d, h, b: scipy.stats.skew(d)),
        "skew_normed": (
            "Skew",
            (0.0, 2.9),
            lambda d, h, b: scipy.stats.skew(d, bias=False),
        ),
        # "mode": ("Mode",
        #        0.0, 3.5,
        #        lambda d, h, b: b[h.argmax()]),
        # "num": ("# cells",
        #        0.0, 2000,
        #        lambda d, h, b: len(d)),
        # "pearson_mode_mean": ("pearson Mode mean",
        #         0.0, 1.2,
        #         joy_plots_of_gradients.pearson_mode_mean_skew),
        # "non_parameteric_skew": ("Non parameteric",
        #         0.0, 0.4,
        #         joy_plots_of_gradients.non_parametric_skew),
        "kurtosis":
        ("Kurtosis", (0.0, 8.0), lambda d, h, b: scipy.stats.kurtosis(d)),
    }

    plot_colors = [  # "mean",
        # "std",
        "cv",
        # "skew",
        # "num",
        # "skew_normed",
        "skew_normed",  # same as pandas
        # "pearson_mode_mean",
        # "non_parameteric_skew",
        # "kurtosis",
    ]

    # basedir = "../../data/bio_film_data/63xdatasets"
    #this_dir = os.path.dirname(__file__)
    this_dir = "/media/nmurphy/BF_Data_Orange/"
    #basedir = os.path.join(this_dir, "../../datasets/LSM700_63x_sigb")
    basedir = os.path.join(this_dir, "datasets/LSM700_63x_sigb")
    # cell_df = pd.read_hdf(os.path.join(basedir, "edge_redo_lh1segment_data_bg_back_bleed.h5"), "cells")
    # cell_df = pd.read_hdf(os.path.join(basedir, "new_edge_bgsubv2_maxnorm_lh1segment.h5"), "cells")
    cell_df = pd.read_hdf(os.path.join(basedir, "single_cell_data.h5"),
                          "cells")
    # cell_df = pd.read_hdf(os.path.join(basedir, "edge_redo_lh1segment_data.h5"), "cells")
    # cell_df = pd.read_hdf(os.path.join(basedir, "lh1segment_bgsub_data.h5"), "cells")
    # cell_df = cell_df[cell_df["area"] > 140]
    cell_df = cell_df[cell_df["distance"] > 2]
    time = 48  # .0
    location = "center"
    file_df = filedb.get_filedb(os.path.join(basedir, "file_list.tsv"))
    strain_map, des_strain_map = strainmap.load()

    # cbar_mins = {0: 0.5, 1:0.0}

    percentile = 0  # 99#
    # green_chan = "meannorm_green"
    # red_chan = "meannorm_red"
    rmax = 6.5
    gmax = 6.5  # 0.4
    green_chan = "green_raw_bg_mean"
    red_chan = "red_raw_bg_mean"
    rmax = 50000
    gmax = 10000
    strains = [
        ("wt_sigar_sigby", red_chan, rmax, "WT\n P$_{sigA}$-RFP"),
        ("wt_sigar_sigby", green_chan, gmax, "WT\n P$_{\mathit{sigB}}$-YFP"),
        (
            "delru_sigar_sigby",
            green_chan,
            gmax,
            "Δ$\mathit{rsbRU}$\n P$_{\mathit{sigB}}$-YFP",
        ),
        (
            "delqp_sigar_sigby",
            green_chan,
            gmax,
            "Δ$\mathit{rsbQP}$\n P$_{\mathit{sigB}}$-YFP",
        ),
    ]
    # ("2xqp_sigar_sigby", green_chan,  gmax,  "2$\\times$rsbQP\n P$_{sigB}$-YFP")]

    fig, ax = plt.subplots(len(plot_colors), len(strains), sharey=True)
    for c, (strain, chan, max_val, name) in enumerate(strains):
        strain_num = des_strain_map[strain]
        distances, sbins, histograms, stats = joy_plots_of_gradients.get_strain_result(
            file_df,
            cell_df,
            time,
            location,
            strain_num,
            chan,
            max_val,
            percentile,
            curve_score_methods,
        )
        for r, k in enumerate(plot_colors):
            color = figure_util.strain_color[strain_num.upper()]
            ax[r, c], mv, leglist = joy_plots_of_gradients.plot_curves(
                ax[r, c], color, distances, sbins, histograms, stats, k)

            if c == len(strains) - 1:
                posn = ax[r, c].get_position()
                cbax = fig.add_axes([
                    posn.x0 + posn.width + 0.0005, posn.y0, 0.015, posn.height
                ])
                label = curve_score_methods[k][0]
                min_zval = curve_score_methods[k][1][0]
                max_zval = curve_score_methods[k][1][1]
                sm = plt.cm.ScalarMappable(
                    cmap=plt.get_cmap("viridis"),
                    norm=plt.Normalize(vmin=min_zval, vmax=max_zval),
                )
                sm._A = []
                _ = plt.colorbar(sm, cax=cbax)  # , fig=fig)
                cbax.set_ylabel(label, rotation=-90, labelpad=8)
                cbax.tick_params(direction="out")

            if r == 0:
                ax[r, c].set_title(name, fontsize=6)
                ax[r, c].get_xaxis().set_ticklabels([])

            ax[r, c].set_xlim(0, max_val)

    # this didnt return the right mode for some reason
    # leg = ax[0, -1].legend(leglist)

    leg = ax[0, -1].legend(leglist, ["Mode", "Mean"],
                           loc="lower left",
                           bbox_to_anchor=(0.84, 0.97))
    leg.set_zorder(400)
    for a in ax.flatten():
        a.tick_params(direction="out")
    ax[0, 0].annotate(
        "Distance from top of biofilm (μm)",
        xy=(0, 0),
        xytext=(0.02, 0.5),
        textcoords="figure fraction",
        # arrowprops=dict(facecolor='black', shrink=0.05),
        horizontalalignment="center",
        verticalalignment="center",
        fontsize="medium",
        color=mpl.rcParams["axes.labelcolor"],
        rotation=90,
    )
    ax[1, 2].annotate(
        "Normalized fluoresence",
        xy=(0, 0),
        xytext=(0.5, 0.04),
        textcoords="figure fraction",
        # arrowprops=dict(facecolor='black', shrink=0.05),
        horizontalalignment="center",
        verticalalignment="center",
        fontsize="medium",
        color=mpl.rcParams["axes.labelcolor"],
    )
    # for a in ax[:, 0].flatten():
    #     ticklabs = a.yaxis.get_ticklabels()
    #     ticklabs = a.get_yticks()#.tolist()
    #     ticklabs[-1] = ''

    letters = ["A", "B", "C", "D", "E", "F", "G", "H", "I", "J"]
    # letter_lab = (-0.13, 0.98)
    for a, l in zip(ax.flatten(), letters):
        a.annotate(
            l,
            xy=(0, 0),
            xytext=(-0.13, 0.95),
            textcoords="axes fraction",
            # arrowprops=dict(facecolor='black', shrink=0.05),
            horizontalalignment="center",
            verticalalignment="center",
            fontsize=figure_util.letter_font_size,
            color="black",
        )
    #    a.text(letter_lab[0], letter_lab[1], l, transform=a.transAxes, fontsize=8)

    filename = "sup_meta_histo"
    width, height = figure_util.get_figsize(figure_util.fig_width_medium_pt,
                                            wf=1.0,
                                            hf=0.6)
    fig.subplots_adjust(left=0.085,
                        right=0.89,
                        top=0.89,
                        bottom=0.13,
                        hspace=0.20,
                        wspace=0.25)
    fig.set_size_inches(width, height)  # common.cm2inch(width, height))
    figure_util.save_figures(fig, filename, ["png", "pdf"], this_dir)
Пример #6
0
def main():

    basedir = os.path.join(this_dir, "../../datasets/LSM700_63x_sigb")

    time = 48
    location = "center"
    # slice_srt, slice_end = 5, 7 #10, 15
    slice_srt_end = (5, 7)

    fig, ax = plt.subplots(2, 2)
    axhisto = ax[1, 1]
    aximage = [ax[0, 0], ax[0, 1], ax[1, 0]]

    for i, (name, path, roi, chans) in enumerate(image_list):
        impath = os.path.join(image_base_dir, path)
        aximage[i] = subfig_draw_bin.get_figure(
            aximage[i],
            name,
            impath,
            roi,
            chans,
            FP_max_min,
            slice_srt_end,
            add_scale_bar=i == 0,
        )
        aximage[i].set_title("")
        aximage[i].text(imgletter_lab[0],
                        imgletter_lab[1],
                        topletters[i],
                        transform=aximage[i].transAxes,
                        **letter_settings)  # , color="white")
        aximage[i].text(0.05,
                        0.05,
                        name,
                        transform=aximage[i].transAxes,
                        **label_settings,
                        color="white")

    #####################
    ## Histograms
    generate_data_subset = False

    strain_map, des_strain_map = strainmap.load()

    file_df = filedb.get_filedb(os.path.join(basedir, "file_list.tsv"))
    cachedpath = os.path.join(basedir, "histo_tops_normed.h5")

    gchan = "green_raw_bg_mean"
    rchan = "red_raw_bg_mean"
    nbins = 150
    gmax = 1
    gbins = np.linspace(0, gmax, nbins)

    list_of_histos = [
        # ("2xqp_sigar_sigby",  gchan, rchan, gbins, slice_srt_end, "2xQP", strain_color["JLB095"]),
        (
            "wt_sigar_sigby",
            gchan,
            rchan,
            gbins,
            slice_srt_end,
            r"WT P$_{\mathit{sigB}}$-YFP",
            strain_color["JLB021"],
        ),
        (
            "delru_sigar_sigby",
            gchan,
            rchan,
            gbins,
            slice_srt_end,
            r"Δ$\mathit{rsbRU}$ P$_{\mathit{sigB}}$-YFP",
            strain_color["JLB088"],
        ),
        (
            "delqp_sigar_sigby",
            gchan,
            rchan,
            gbins,
            slice_srt_end,
            r"Δ$\mathit{rsbQP}$ P$_{\mathit{sigB}}$-YFP",
            strain_color["JLB039"],
        ),
    ]
    axes = [axhisto] * len(list_of_histos)
    if generate_data_subset:
        df = pd.read_hdf(os.path.join(basedir, "single_cell_data.h5"), "cells")
        cellsdf = subfig_normalised_histos.get_data_subset(
            df, file_df, list_of_histos, time, location, cachedpath)
    else:
        cellsdf = pd.read_hdf(cachedpath, "cells")

    axes = subfig_normalised_histos.get_figure(cellsdf, file_df, axes, time,
                                               location, list_of_histos)
    axes[0].legend()

    axhisto.text(hisletter_lab[0],
                 hisletter_lab[1],
                 letters[0],
                 transform=axhisto.transAxes,
                 **letter_settings)

    axhisto.set_ylabel("Percentage of cells")

    axhisto.set_xlim(0, gmax)
    axhisto.set_ylim(0, 8.5)
    axhisto.tick_params(axis="x", which="both",
                        direction="out")  # , length=2, pad=0)
    axhisto.tick_params(axis="y", which="both",
                        direction="out")  # , length=2, pad=0)
    axhisto.yaxis.set_major_locator(mticker.MaxNLocator(nbins=3, integer=True))
    axhisto.set_xlabel("Normalised cell fluorecence")

    filename = "demo_longtail"
    fig.subplots_adjust(left=0.05,
                        right=0.95,
                        top=0.99,
                        bottom=0.1,
                        hspace=0.08,
                        wspace=0.20)
    width, height = figure_util.get_figsize(figure_util.fig_width_small_pt,
                                            wf=1.0,
                                            hf=0.9)
    fig.set_size_inches(width, height)
    figure_util.save_figures(fig, filename, ["png", "pdf"], this_dir)
Пример #7
0
def main():
    this_dir = os.path.dirname(__file__)
    basedir = os.path.join(this_dir, "../../datasets/LSM700_63x_sigb")
    #cell_df = pd.read_hdf(os.path.join(basedir, "edge_redo_lh1segment_data_bg_back_bleed.h5"), "cells")
    cell_df = pd.read_hdf(os.path.join(basedir, "single_cell_data.h5"), "cells")
    print(cell_df.columns)

    file_df = filedb.get_filedb(os.path.join(basedir, "file_list.tsv"))
    file_df.loc[file_df["time"] == 26.0, ['time']] = 24.0
    file_df.loc[file_df["time"] == 38.0, ['time']] = 36.0
    
    USE_CACHE_PLOTS = False


    time = 48
    location = "center"
    slice_srt, slice_end = 5, 7 

    fig, axhisto = plt.subplots(1, 1)

    strain_map, des_strain_map = strainmap.load()
    gchan = "green_raw_bg_autofluor_bleedthrough_meannorm"

    gmax_val = 20
    nbins=150

    gbins = (0, gmax_val, nbins)

    percentile = 0
    list_of_histos = [ 
            ("wt_sigar_sigby", gchan, "WT P$_{sigB}$-YFP", strain_color["JLB021"]),
            ("delqp_sigar_sigby", gchan, "ΔrsbQP P$_{sigB}$-YFP", strain_color["JLB039"]),
            ("delru_sigar_sigby", gchan, "ΔrsbRU P$_{sigB}$-YFP", strain_color["JLB088"]),
            ("2xqp_sigar_sigby", gchan, "2$\\times$rsbQP P$_{sigB}$-YFP", strain_color["JLB095"]),
    ]
    print("-----------")
    lelines = []
    lelabs = []
    for i, (strain, chan, label, color) in enumerate(list_of_histos):
        print(label)
        fids = file_df[(file_df["time"] == time) &
                    (file_df["location"] == location) &
                    (file_df["strain"] == des_strain_map[strain])].index
        strain_df = cell_df[cell_df["global_file_id"].isin(fids)]
        #strain_df = get_strain(file_df, cell_df, strain) 
        plot_args = {"color":color, "max_min":"none", "mode_mean":False}
        tbins = gbins
        dset = time, location, strain

        args = (axhisto, strain_df, chan, tbins, (slice_srt, slice_end), dset, percentile, USE_CACHE_PLOTS, this_dir, plot_args)
        axhisto, line, _ = subfig_indivfile_histo.get_figure(*args)
        lelines += [line]
        lelabs += [label]
    axhisto.legend(lelines, lelabs)
        
    axhisto.set_xlabel("Normalised cell fluorecence (bleed through subtracted)")

    axhisto.set_ylabel("Percentage of cells") 
    axhisto.set_ylim(0, 7)
    axhisto.set_xlim(0, gmax_val)
        

    filename = "sup_bleed_histo"
    fig.subplots_adjust(left=0.1, right=0.9, top = 0.98, bottom=0.2)#, hspace=0.35, wspace=0.2)
    width, height = figure_util.get_figsize(figure_util.fig_width_small_pt, wf=1.0, hf=0.5)
    fig.set_size_inches(width, height)# common.cm2inch(width, height))

    figure_util.save_figures(fig, filename, ["png", "pdf"], this_dir)