Bilateral adrenalectomy forces the patient to undergo glucocorticoid replacement therapy and bear a lifetime risk of adrenal crisis. Adrenal autotransplantation is considered useful to avoid adrenal crisis and glucocorticoid replacement therapy. However, the basic process of regeneration in adrenal autografts is poorly understood. Here, we investigated the essential regeneration factors in rat adrenocortical autografts, with a focus on the factors involved in adrenal development and steroidogenesis, such as Hh signalling. A remarkable renewal in cell proliferation and increase in Cyp11b1, which encodes 11-beta-hydroxylase, occurred in adrenocortical autografts from 2–3 weeks after autotransplantation. Serum corticosterone and adrenocorticotropic hormone levels were almost recovered to sham level at 4 weeks after autotransplantation. The adrenocortical autografts showed increased Dhh expression at 3 weeks after autotransplantation, but not Shh, which is the only Hh family member to have been reported to be expressed in the adrenal gland. Increased Gli1 expression was also found in the regenerated capsule at 3 weeks after autotransplantation. Dhh and Gli1 might function in concert to regenerate adrenocortical autografts. This is the first report to clearly show Dhh expression and its elevation in the adrenal gland.
The adrenal gland comprises the adrenal cortex and the medulla. In humans, the adrenal cortex is composed of three anatomical layers namely the zona glomerulosa (ZG), zona fasciculata (ZF), and zona reticularis. In the rat adrenal cortex, aldosterone synthase (Cyp11b2) in ZG and 11-beta-hydroxylase (Cyp11b1) in ZF catalyse the production of aldosterone and corticosterone, respectively. These CYP genes are regulated by NR5A1 (also known as SF1 or Ad4BP)1. There is also an area with no expression of Cyp11b1 and Cyp11b2 termed the undifferentiated zone (ZU) located between ZG and ZF in rats2,3,4.
Familial phaeochromocytoma patients, such as those with multiple endocrine neoplasia type 2, may require bilateral adrenalectomy, after which the patients need to take glucocorticoid replacement therapy throughout their life5. Moreover, the risk of adrenal crisis, a life-threatening event, remains as long as the patients live6. Therefore, partial adrenalectomy may be performed as an adrenal sparing surgery to avoid adrenal crisis5. However, there is the risk that phaeochromocytoma may recur from the ipsilateral residual adrenal gland even after partial adrenalectomy7. In this case, autotransplantation of the adrenal cortex may reduce the risk of phaeochromocytoma recurrence8 because the adrenal medulla, which is regarded as the origin of phaeochromocytoma, does not regenerate, whereas adrenocortical cells can be regenerated in adrenal autografts in animal models9. Adrenal transplantation was studied in animals even in the early 1900s10; to our knowledge, the oldest reported adrenal transplantation was conducted in a patient with Addison’s disease in 192211. Establishment of adrenocortical autotransplantation has the advantage of reducing recurrence risk and eliminating the need for glucocorticoid replacement therapy in familial phaeochromocytoma patients8. However, the success rate for adrenal autotransplantation in humans is low, ranging from 20 to 35%12,13 in contrast to animal models14,15. Consequently, to clarify the regeneration step of adrenocortical autografts after transplantation, and the factors affecting their remodelling and regeneration, analysis of adrenocortical autografts in animal models is required.
Although adrenocortical autotransplantations have been successful in rodents14,15, the underlying mechanism has not been clarified yet. Several patterns of adrenocortical cell zonation, renewal, and remodelling under various conditions have been reported2,16,17. Apparently, pools of stem/progenitor cells exist in the adrenal capsule, the subcapsular, and other regions of the adrenal gland2,18. It is well-known that SHH plays a key role in adrenal development and is localised in the subcapsular region of mice and in the ZU of rats3,18,19. Shh(+) cells have also been identified as stem/progenitor cells2,18,19,20. To date, only Shh has been reported to be expressed in the adrenal gland among the Hh family members2. SHH regulates Gli1, the effector of Hh signalling and a determinant of cell fate during embryonic development21. Gli1(+) cells have also been identified as stem/progenitor cells and are localised in the adrenal capsule22. In addition, SHH(+) and GLI1(+) progenitor cells differentiate into steroidogenic cells. It is conceivable that the Hh signalling pathway is involved in the regeneration process of adrenocortical autografts as in the development of the adrenal cortex. In this study, we examined whether Hh signalling functions as a remodelling and/or regeneration factor for adrenocortical autografts. Unexpectedly, we found that Shh was suppressed and Dhh was upregulated in the regeneration step of rat adrenocortical autografts. Our study clearly demonstrates Dhh expression in the adrenal gland for the first time.
Enlargement of adrenocortical autografts
Macroscopically (Supplementary Fig. 1), we identified the adrenocortical autograft as a yellowish mass throughout the post-operative period. Adrenocortical autografts showed thin shapes at post-operative day (POD) 7 (Supplementary Fig. 1). At two weeks after surgery, almost all adrenocortical autografts were flat-shaped and fragile to handle in all rats (Supplementary Fig. 1). After three weeks (Supplementary Fig. 1), the autografts were stable and increased in size compared to POD14. There was no difference between POD21 and POD28 with respect to gross appearance.
Haematoxylin and eosin (HE) staining showed (i) partial loss of adrenocortical cells, (ii) a few remnant adrenocortical cell clusters around the capillaries, and (iii) stromal-like cell proliferation from POD7 to POD14 (Fig. 1). At POD21, we easily identified the arrangement of the renewing adrenocortical cells in the cord-like structures similar to the normal ZF (Fig. 1). These cord-like structures were completely encapsulated in the renewal capsule and in the columns directed towards the veins (Supplementary Fig. 2). Indeed, a prominent increase in adrenocortical cells was observed in the region encapsulated within the capsule after POD16 (Fig. 1 and Supplementary Fig. 2). Four weeks after surgery, HE staining indicated fully formed adrenocortical cells (Fig. 1).
Autotransplanted rats recover from Adrenocortical insufficiency at POD21
Serum corticosterone (ng/ml) showed a significant reduction at POD7 (n = 4, mean ± standard error; 32.6 ± 5.3, p = 0.002, r = 0.74) and POD14 (n = 4, 78.4 ± 8.0, p = 0.008, r = 0.67) compared to the sham group (n = 10, 246.9 ± 33.5) (Fig. 2A). There was a gradual increase in the level of serum corticosterone. There was no significant difference between the sham group and POD21 (n = 4, 164.9 ± 13.7) or the sham group and POD28 (n = 4, 206.4 ± 28.8). On the other hand, serum adrenocorticotropic hormone (ACTH) (pg/ml) showed a significant increase at POD7 (n = 4, mean ± standard error; 215.3 ± 103.7, p = 0.004, r = 0.72) and POD14 (n = 4, 197.1 ± 55.7, p = 0.004, r = 0.72) compared to the sham group (n = 10, 17.1 ± 6.2) (Fig. 2B). There was no significant difference between the sham group and POD21 (n = 4, 44.1 ± 23.9) or the sham group and POD28 (n = 4, 63.8 ± 17.5).
To clarify the recovery of the adrenocortical insufficiency in adrenal autografts, the correlations between corticosterone and ACTH were analysed at each time point (Fig. 2C–G). A significant negative correlation was found between corticosterone and ACTH at POD28 (r = 0.86, p < 0.05) (Fig. 2G). Although normal values of serum corticosterone and improvement of the hyperactive hypothalamic-pituitary-adrenal axis were found at POD28, latent adrenocortical insufficiency was suggested at POD28 based on the negative correlation.
Increase in Cyp11b1 (+) cells in adrenocortical autografts
To confirm the evidence of functional recovery, we examined Cyp11b1 expression in adrenocortical autografts using the RNAscope/Basescope technique.
RNAscope is a novel RNA in situ hybridisation analysis using a unique double-Z design probe23. The design helps to increase the sensitivity and specificity for target gene expression. RNAscope signals show as dots, with each dot corresponding to a single mRNA copy23.
Cyp11b1 staining in the adrenal gland of a sham-operated rat using the Basescope showed a relatively strong expression in the ZF and a gradually decreasing expression towards the inner medulla (Fig. 3A). In adrenocortical autografts at POD7 and POD14, remnant adrenocortical cells around the capillary circumference showed strong Cyp11b1 expression (Figs 4A and 5A). There was no signal in the autografts except for remnant adrenocortical cells at POD7 and POD14 (Figs 4A and 5A). Diffuse Cyp11b1 expression over the adrenocortical autograft was recognised at POD21 (Fig. 6A), and the expression level per cell was lower than that in the adrenocortical autograft at POD28 (Fig. 7A). At POD28, Cyp11b1 was expressed in a polarised manner, which is similar to its expression pattern in the adrenal gland of sham-operated rats, and a strong Cyp11b1 expression was detected in the regenerated ZF-like region just beneath the renewing capsular region (Fig. 7A).
Recovery of Cyp11b1 and absence of Cyp11b2/CYP11B2 in adrenocortical autografts
To confirm the expression of Cyp11b1 and Cyp11b2 in whole adrenocortical autografts, we conducted digital mRNA counts using nCounter technology (Fig. 2H,I). The Rattus Cyp11b1 (Acc#: NM_012537.3) sequence contains several deletions compared with the Rattus Cyp11b2 sequence (NM_012538.2); therefore, we created a unique probe against Rattus Cyp11b2, but we could not create a unique probe for Cyp11b1, because the homology among Rattus Cyp11b1, Cyp11b2 (94% identity against Cyp11b1), Cyp11b3 (NM_181824.1, 94% identity), and Cypxib1 (XM_017595365.1) is very high.
No expression of Cyp11b2 was found with the specific Cyp11b2 probe in adrenocortical autografts (mean ± standard deviation, 76.4 ± 76.1 at POD7, 19.7 ± 5.6 at POD14, 117.4 ± 152.9 at POD21, 8.8 ± 5.8 at POD28) (Fig. 2I), as less than 120 counts with the Cyp11b2 probe are considered negative depending on the background counts. Cyp11b2 was expressed in the sham-operated adrenal gland (357.2 ± 310.4 at POD7, 3506.6 ± 754.0 at POD14, 4268.8 ± 1133.9 at POD21, 3758.7 ± 781.1 at POD28). Saline supplementation might have suppressed the Cyp11b2 expression at POD7 (see Materials and Methods). In contrast, the Cyp11b1 probe in nCounter detected a significant reduction in cytochrome P450 11B mRNAs in the autografts (17313.8 ± 5046.9) compared with that in sham animals (146606.1 ± 19691.6) at POD7 (p = 0.021, r = 0.82) and demonstrated upregulation of cytochrome P450 11B mRNAs in the autografts (236321.2 ± 20738.8) compared with that in sham animals (131732.2 ± 29101.7) at POD14 (p = 0.021, r = 0.82) (Fig. 2H). We had estimated that Cyp11b1 expression was decreased at POD7 and POD14, which reflected a loss of adrenocortical cells as determined using the Basescope. However, Cyp11b1 expression did not result in a gradual increase in serum corticosterone levels and had a transient peak at POD14, suggesting that the nCounter Cyp11b1 probe might have detected other cytochrome P450 11B mRNAs. At POD21, there was no significant difference in the detection of the nCounter Cyp11b1 probe between the autografts (128927.5 ± 14906.7) and sham animals (147918.0 ± 12235.6). The nCounter Cyp11b1 probe detected a significant increase in cytochrome P450 11B mRNAs in the autografts (283069.0 ± 29285.4) compared with that in sham animals (132757.8 ± 24891. 9) at POD28 (p = 0.021, r = 0.82).
To examine the presence of ZG cells in the adrenocortical autograft, we immunohistochemically stained for rattus ZG specific markers, CYP11B2 and DAB224,25. CYP11B2 staining in the adrenal gland of a sham-operated rat showed a strong expression in the ZG (Fig. 3B). The absence of CYP11B2 was observed in the adrenocortical autograft as well as the results of nCounter (Figs 4B–7B). However, DAB2 signals were detected not only in the ZG of sham rat, but also in remnant adrenocortical cells at POD7 and POD14 and in the subcapsular region at POD21 and POD28 (Figs 3C–7C).
Adrenocortical autograft cell proliferation occurs in subcapsular region
To identify the cell proliferation in adrenal autografts, proliferating cell nuclear antigen (PCNA) staining was performed. Cell proliferation has been reported to be dominant in ZG in the adrenal gland,26 and PCNA signals in adrenal cortex with sham operation were also found in ZG (Fig. 3D). At POD7 and POD14, PCNA was broadly and sparsely observed in autografts (Figs 4D and 5D). PCNA was detected in subcapsular region again at POD21 and POD28 (Figs 6D and 7D).
Upregulation of Dhh in adrenocortical autografts
In the adrenal cortex of sham-operated rats, RNAscope findings for Gli1 and Shh, which were detected in the adrenal capsule and in the ZU, respectively (Fig. 3E,F), were consistent with a previous report27. Gli1 was expressed in stromal cells adjacent to the remnant adrenocortical cells at POD7 and POD14 (Figs 4E and 5E). Gli1 expression sites were changed to renewal capsular cells and adrenocortical cells close to the capsule at POD21 (Fig. 6E). Gli1 expression at POD28 was decreased in the renewal capsular region compared to that at POD21 (Figs 6E and 7E), and persisted in the adrenocortical cells in the subcapsular region at POD28 (Fig. 7E). We did not detect any Shh expression through POD7–21 (Figs 4F–6F). We detected a few Shh signals in the regenerated adrenocortical cells at POD28 (Fig. 7F). In contrast, Dhh was remarkably and diffusely expressed in the renewal adrenocortical cells at POD21 compared to the sham-operated adrenal gland (Figs 3G and 6G). A few Dhh expression signals were detected at POD7 and POD14 (Figs 4G and 5G). Dhh showed scattered expression in both the adrenal cortex with sham operation and adrenocortical autografts at POD28 (Fig. 7G). In contrast to Dhh expression, few Ihh expression was detected in the adrenal gland upon sham operation and in adrenocortical autografts. There was also no change throughout the regeneration period (Figs 3H–7H).
The dim cytoplasmic fluorescence signals were regarded as autofluorescence of adrenocortical cells (Supplementary Fig. 3). We used unmixing analysis for extracting autofluorescence (Supplementary Fig. 4 and method section).
A few Wt1(+) Gli1(+) cells in adrenocortical autografts
WT1 has been reported as a direct regulator of Gli1 without Hh input in the adrenal gland28. To clarify the involvement of WT1 in regulating Gli1 in the adrenocortical autograft, double staining with Wt1 (FastGreen) and Gli1 (FastRed) was conducted using RNAscope (Fig. 8). In the adrenal glands of sham-operated rats, Wt1 expression was found to be weak in the capsule and cortex, and Gli1 was located in the capsule (Fig. 8). Some blurred blue signals in adrenal cells were regarded as background based on negative control study (Fig. 8). From POD7 to POD21, we found Wt1 expression around the capillaries, Gli1 expression adjacent to Wt1, and a few Wt1(+) Gli1(+) cells (Fig. 8). Wt1 was suppressed at POD14 and its expression was increased again around the veins at POD21 (Fig. 8). At POD28, Wt1 was re-suppressed around the veins and slightly expressed in renewal adrenocortical cells (Fig. 8).
HE staining of adrenocortical autografts showed loss of most adrenocortical cells by 1 week after operation. The dynamic changes, dependent on the regeneration step, occurred between 2 and 3 weeks after surgery as reported previously9,15,29. After four weeks, the adrenocortical autografts showed morphological and functional recovery as shown by the restoration of serum corticosterone levels with no statistical difference compared to sham animals. We also found strong expression of Dhh and Gli1 during the remodelling and regeneration process in adrenocortical autografts.
Differentiated ZG cells are known to undergo lineage conversion into ZF cells15,16. ZG-specific gene deletion of Nr5a1 prevents lineage conversion into ZF cells, but the production of functional ZF cells is maintained16. These results suggest that ZF cells are produced from ZG cells as well as from other cell populations. There was no obvious ZG in the autograft at POD21 and POD28 based on our Cyp11b1 and Cyp11b2/CYP11B2 expression analysis with immunohistochemistry (IHC), in situ hybridisation, and the nCounter method. The Cyp11b1 expression pattern in the Basescope analysis and the lack of Cyp11b2/CYP11B2 expression in IHC and the nCounter analysis indicated that almost all the regenerated adrenocortical cells were ZF cells. Cell proliferation has been shown dominantly in both mouse ZG26 and ZF in rat enucleation models of the adrenal gland30. In the present study, PCNA (+) cells were increased at POD7 and POD14, and strong PCNA (+) cells were located in the subcapsular region at POD21 and POD28. These findings were consistent with a previous report31. These regenerated adrenocortical cells in the subcapsular region might be directly differentiated into Cyp11b1-expressing cells in the adrenocortical autografts without the lineage conversion from ZG cells.
Although no CYP11B2 was found at POD7 and POD14 indicating the absence of ZG cells, strong DAB2 signals were found in those periods. Absence of ZG in adrenocortical autograft was also previously reported32. DAB2 has multifaceted roles and is expressed in epithelial cells of several tissues33. DAB2 is also induced by physiological stimulations34. In addition, it is known that CYP11B2 expression is restricted to a limited number of ZG cells expressing DAB2 in humans35. Therefore, there might be a dissociation between CYP11B2 and DAB2 in adrenal cortex remodelling. We observed DAB2 expression in remnant adrenocortical cells at the early stages. However, subcapsular localisation of DAB2 was found on POD21. It could be said that immature ZG cells without CYP11B2 might be regenerated from POD21 onwards.
Not surprisingly, overall Gli1 expression was observed in the adrenocortical autograft similar to the developmental stage, suggesting the participation of Hh signalling in the regeneration of adrenocortical autografts. The expression was prominent at POD21. Although Shh (+) Gli1 (+) progenitor cells have been reported to differentiate into steroidogenic cells in the canonical process18, we observed only slight expression of Shh in the adrenocortical autografts with no correlation between Shh and Gli1 expression in the adrenocortical autografts. We then performed RNAscope analysis with other Hh signalling ligands, Dhh and Ihh. Expression of Ihh was hardly found and showed no change in all the experiments. In contrast, Dhh showed strong and diffused expression in the regenerating adrenocortical cells at 3 weeks after the operation. DHH but not SHH might be one of the key regulators of GLI1 in adrenocortical autografts as in gonads21,36,37, and the upregulation of Dhh implies its importance for the regeneration of adrenocortical autografts.
It is well known that WT1 directly controls Gli1 transcription in the adrenal primordia without Hh signalling28 and that it is implicated in steroidogenic cell differentiation in both the adrenal cortex and the gonads28,38. Moreover, WT1 is a tumour suppressor gene and is related to the distant metastasis and progression of tumour cells by its function as a master regulator of the mesenchymal-epithelial transition and epithelial-mesenchymal transition39. WT1 is highly expressed in the blood vessels of most human tumours but not in the blood vessels in normal tissues40,41. In this study, no increase in Wt1 expression was found in the mesenchyme of normal muscle tissues at the site of transplantation or in the remnant autografted adrenal tissues at POD7. However, WT1 could be involved in graft vascularisation, as a highly specific expression of Wt1 was observed in the perivascular regions in autografts at POD7. Interestingly, an alternative splice variant, WT1-KTS, is known to stimulate the expression of the receptor for the vascular endothelial growth factor, Kdr, in murine embryonic gonads42, and a high Kdr expression was observed in a previous study on adrenocortical autografts43. Accordingly, regulation of vascularisation by WT1 was considered as one of the key factors for the regeneration step of adrenocortical autografts at the initial stage.
In conclusion, an increase in Dhh and Gli1 expression was observed during the regeneration of adrenocortical tissues. WT1 was suggested to contribute to the regeneration of blood vessels and synergistically potentiate DHH effect. This report is the first to clearly demonstrate the expression of Dhh and its elevation in the adrenal gland. To clarify whether DHH directly affects adrenocortical regeneration, further autotransplantation studies using Dhh knockout strains with genome editing will need to be conducted.
Materials and Methods
In total, 37 male Wistar rats (age, 7 weeks; weight, 210–270 g) were purchased from Shimizu Laboratory Supplies (Kyoto, Japan) and housed in a sound-attenuated light-controlled room (lights on at 8:00 a.m. and off at 8:00 p.m.; 12 h light-dark cycle; constant environment at 25 ± 1 °C and 50 ± 10% relative humidity) for 2 weeks before the operation. Food and water were provided ad libitum. All animal experiments were approved by the Ethics Committee on Animal Experiments at Kansai Medical University (approval ID: 17-051) and were conducted in accordance with the Guide for the Care and Use of Laboratory Animals of the Institute for Laboratory Animal Research.
Adrenocortical autotransplantation was performed in 9-week-old rats as described previously44. Briefly, bilateral adrenal glands were resected under general anaesthesia by inhalation of 2% isoflurane (Pfizer Japan Inc., Tokyo, Japan) and 3 L/minute oxygen. The adrenal gland was divided into four pieces and the medulla was discarded. The adrenocortical autografts retaining the capsule, ZG, and ZU4 were autotransplanted into the right biceps femoris. Sham operations without adrenalectomy were performed simultaneously. The animals could survive on saline without any glucocorticoid replacement following the adrenalectomy45. We then performed blood collection from the rat heart and tissue sampling at the following designated periods. Sera were isolated by centrifugation at 1,500 × g for 30 min at 4 °C and stored at −80 °C until use.
Adrenal tissues were immersion-fixed overnight in 4% formaldehyde in phosphate-buffered saline (PBS), and frozen tissues, embedded in OCT compound, were cut into 10 µm-thick sections. Each 10 µm-thick frozen section was hydrated and stained with HE according to the general method.
The procedure of fixing and sectioning were the same as the procedure in the section above. Heat-induced epitope retrieval was conducted with 10 mM Tris-HCl (pH 6.0) for 5 min for PCNA and DAB2 staining. Inactivation of endogenous peroxidases with 0.1% phenylhydrazine in PBS was performed for 30 min. Sections were then incubated with mouse anti-PCNA antibody (610664, BD biosciences, CA, USA; dilution at 1:1000) with PBS containing 0.3% triton X-100 or mouse anti-Disabled-2/p96 antibody (610464; BD biosciences, CA, USA; dilution at 1:1000) with PBS containing 0.3% triton X-100 overnight at room temperature. After washing with PBS containing 0.3% triton X-100, sections were incubated with ImmPRESS REAGENT anti-mouse IgG (MP-7422; VECTOR LABORATORIES, INC., CA, USA) for 30 min, followed by staining with diaminobenzidine. Sections were counterstained with haematoxylin.
For CYP11B2, heat-induced epitope retrieval step was omitted. After inactivation of endogenous peroxidases, sections were blocked with 10% goat serum and 0.5% SDS in 0.1 M Tris pH 7.4 for 1 h. Then, sections were incubated with rabbit anti-CYP11B2 antibody24 (dilution 1:6000 with 0.1 M Tris, 10% goat serum and 0.2% Tween-20) supplied by C. Gomez-Sanchez (University of Mississippi Medical Center) overnight at room temperature. After washing with PBS containing 0.2% Tween-20, sections were incubated with goat anti-rabbit IgG-Alexa flour 488 for 1 h (A27034; Thermo Fisher Scientific, MA, USA; dilution 1:1000 with 0.1 M Tris, 10% goat serum and 0.2% Tween-20).
Control experiments with omission of the antibodies were conducted to extract the reference spectral profile.
Enzyme immunoassay for serum corticosterone and ACTH levels
We measured the rat serum corticosterone and ACTH levels in duplicate using a Corticosterone EIA Kit (YK240; Yanaihara Institute Inc., Shizuoka, Japan) and an ACTH ELISA kit (M046006; MD bioproducts, Zurich, Switzerland) following the manufacturer’s protocol, respectively. The range of detection for the corticosterone concentration was from 0.21 to 50 ng/mL and for ACTH concentration was from 1.0 to 640 pg/ml, respectively. The intra-assay coefficient of variation and inter-assay coefficient of variation were 2.5–4.7% and 7.7–9.8% in Corticosterone EIA Kit and 2.24–6.71% and 6.9–7.1% in ACTH ELISA kit, respectively.
RNAscope and Basescope (in situ hybridisation)
Adrenal tissues were treated according to the Sample Preparation Technical Note for Fixed Frozen Tissue (ACD, Hayward CA, USA). In brief, fixed frozen tissues embedded in OCT compound were cut into 10 µm-thick sections and mounted on Superfrost Plus slides (Fisher Scientific, Waltham MA, USA) for RNA in situ hybridisation. These sections were air-dried at −20 °C and stored at −80 °C until use.
We performed RNAscope analysis with rat probes (Supplementary Table 1) to reveal the mRNA expression and localisation in adrenocortical autografts using the BaseScope Reagent Kit, RNAscope 2.5HD Reagent Kit (Single-plex, RED), or RNAscope 2-plex Reagent Kit (ACD) with the HybEZ Hybridisation system according to the kit manual. Each mRNA was detected with FastRed or FastGreen. Counterstaining was conducted with 33% Mayer’s haematoxylin or 50% Gill’s haematoxylin.
Direct count of mRNA copies
Adrenal glands of sham-operated rats and adrenocortical autografts were quickly removed. The removed adrenal tissues were isolated from the surrounding fat and muscle tissues as much as possible, and total RNA was extracted using Sepasol-RNA I Super G reagent (Nacalai Tesque, Inc., Kyoto, Japan). Cyp11b1 and Cyp11b2 mRNAs in each sample were hybridised with the target probes (Supplementary Table 2) and reporter tags (Elements XT TagSet system, NanoString Technologies, Inc. N Seattle, WA). After trapping, the RNA copy number was counted in a digital analyser with the nCounter system (NanoString Technologies, Inc. N Seattle, WA) according to the provided manual. We analysed the data using nSolver analysis software (NanoString Technologies, Inc. N Seattle, WA). Each mRNA count was normalised to Hprt1 as the internal control gene. Background subtraction was performed using the raw counts of RNase-free water.
Optical images were collected using ECLIPSE E1000M (Nikon, Tokyo, Japan), ECLIPSE Ci (Nikon, Tokyo, Japan), or LSM700 (ZEISS, Oberkochen, Germany) microscopes. Autofluorescence frequency interferes with the identification of specific signals in fluorescence imaging and varies in each organ46. Some autofluorescence are derived from endogenous molecules related to metabolism, such as nicotinamide adenine dinucleotide phosphate, and lipofuscin46,47,48. Therefore, autofluorescence has been reported to be useful for monitoring metabolic changes48. The adrenal gland is one of the organs known to produce autofluorescence47. We found autofluorescence in the adrenal gland and adrenocortical autograft tissues (Supplementary Fig. 3). Recently, “unmixing” technique by spectral imaging was reported to separate desired signals from autofluorescence49. The autofluorescence spectral profile in adrenocortical cells could be clearly discriminated from the fluorescence with FastRed chromogen by RNAscope and from the fluorescence with Alexa 488 green fluorophore profile using lambda mode and spectral unmixing algorithms equipped with Zeiss LSM700 microscope. The autofluorescence spectral profile, as a reference, was extracted from the control experiments described above (Supplementary Fig. 4). Positive signal spectral profile of the fluorescence with FastRed chromogen in RNAscope was extracted from ovary tissues (Supplementary Fig. 4). For all the fluorescence images, we subtracted the autofluorescence from the original figures by linear unmixing.
Normality was analysed by the Shapiro-Wilk normality test for all groups.
The distributions of the Cyp11b1 and Cyp11b2 expression levels via nCounter technology were compared between the sham and autograft groups at each time point using the Mann-Whitney U-test because the data from one group were not normally distributed (P < 0.05). P < 0.05 was considered to indicate a statistically significant difference in each comparison of gene expression. The distributions of corticosterone and ACTH concentrations between the sham and autograft groups were compared using ANOVA and the Mann-Whitney U test using SPSS for Windows. Significance levels were set at p < 0.0125 for corticosterone and ACTH concentrations after Bonferroni’s correction for multiple comparisons. The correlations between corticosterone and ACTH concentrations at each time were examined using the Spearman correlation coefficient test. A p value less than 0.05 was considered as statistically significant.
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The present study was supported by the Japan Society for the Promotion of Science KAKENHI fund (Grant Number 15K08224 and 16K08533 to ST, Grant Number 16K10483 to TY), a research grant from Yamaguchi Endocrine Research Foundation and Kansai Medical University to NT, and a MEXT-Supported Program for the Strategic Research Foundation at Private Universities (Grant Number S1101034 and S1201038) to HY. The authors would like to thank the Department of Pathology at Kansai Medical University and Prof. Kiyoshi Kurokawa (Osaka International University) for their helpful comments, and the Central Research Center and Kansai Medical University research consortium for their support. We thank Ms. Ayako Nagata for providing technical assistance.
The authors declare no competing interests.
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Takizawa, N., Tanaka, S., Oe, S. et al. Involvement of DHH and GLI1 in adrenocortical autograft regeneration in rats. Sci Rep 8, 14542 (2018) doi:10.1038/s41598-018-32870-9