Mammalian Heat Shock Factor 1 Is Essential for Oocyte Meiosis and Directly Regulates Hsp90α Expression

Heat shock transcription factor 1 (HSF1) is the main regulator of the stress response that triggers the transcription of several genes encoding heat shock proteins (Hsps). Hsps act as molecular chaperones involved in protein folding, stability, and trafficking. HSF1 is highly expressed in oocytes and Hsf1 knock-out in mice revealed that in the absence of stress this factor plays an important role in female reproduction. We previously reported that Hsf1-/- females produce oocytes but no viable embryos. Consequently, we asked whether oocytes require HSF1 to regulate a particular set of Hsps necessary for them to develop. We find that Hsp90α (Hspaa1) is the major HSF1-dependent chaperone inasmuch as Hsf1 knock-out resulted in Hsp90-depleted oocytes. These oocytes exhibited delayed germinal vesicle breakdown (or G2/M transition), partial meiosis I block, and defective asymmetrical division. To probe the role of Hsp90α in this meiotic syndrome, we analyzed meiotic maturation in wild-type oocytes treated with a specific inhibitor of Hsp90, 17-allylamino-17-demethoxy-geldanamycin, and observed similar defects. At the molecular level we showed that, together with these developmental anomalies, CDK1 and MAPK, key meiotic kinases, were significantly disturbed. Thus, our data demonstrate that HSF1 is a maternal transcription factor essential for normal progression of meiosis. Heat shock transcription factor 1 (HSF1) is the main regulator of the stress response that triggers the transcription of several genes encoding heat shock proteins (Hsps). Hsps act as molecular chaperones involved in protein folding, stability, and trafficking. HSF1 is highly expressed in oocytes and Hsf1 knock-out in mice revealed that in the absence of stress this factor plays an important role in female reproduction. We previously reported that Hsf1-/- females produce oocytes but no viable embryos. Consequently, we asked whether oocytes require HSF1 to regulate a particular set of Hsps necessary for them to develop. We find that Hsp90α (Hspaa1) is the major HSF1-dependent chaperone inasmuch as Hsf1 knock-out resulted in Hsp90-depleted oocytes. These oocytes exhibited delayed germinal vesicle breakdown (or G2/M transition), partial meiosis I block, and defective asymmetrical division. To probe the role of Hsp90α in this meiotic syndrome, we analyzed meiotic maturation in wild-type oocytes treated with a specific inhibitor of Hsp90, 17-allylamino-17-demethoxy-geldanamycin, and observed similar defects. At the molecular level we showed that, together with these developmental anomalies, CDK1 and MAPK, key meiotic kinases, were significantly disturbed. Thus, our data demonstrate that HSF1 is a maternal transcription factor essential for normal progression of meiosis. In mammals there are several heat shock factors (HSF1, -2, and -4) 3The abbreviations used are: HSF, heat shock factor; Hsp, heat shock protein; ChIP, chromatin immunoprecipitation; MII, metaphase II; GVBD, germinal vesicle (GV) breakdown; 17AAG, 17-(allylamino)-17-demethoxygelda-namycin; MEK, mitogen-activated protein kinase/extracellular signal-regulated kinase kinase; IBMX, isobutylmethylxanthine; ERK, extracellular signal-regulated kinase; MAPK, mitogen-activated protein (MAP) kinase; ERK1/2-P, ERK1/2 phosphorylated forms; qPCR, quantitative PCR. that share a similar DNA binding domain, but HSF1 appears to be the major transcriptional regulator responsible for the stress-inducible expression of heat shock proteins (Hsps) (1Pirkkala L. Nykanen P. Sistonen L. FASEB J. 2001; 15: 1118-1131Crossref PubMed Scopus (814) Google Scholar, 2Christians E.S. Benjamin I.J. Handb. Exp. Pharmacol. 2006; : 139-152Crossref PubMed Scopus (3) Google Scholar). The Hsf1 gene was targeted by homologous recombination in murine ES cells, and Hsf1 knock-out mice were produced by three different laboratories (3Xiao X. Zuo X. Davis A.A. McMillan D.R. Curry B.B. Richardson J.A. Benjamin I.J. EMBO J. 1999; 18: 5943-5952Crossref PubMed Scopus (446) Google Scholar, 4Zhang Y. Huang L. Zhang J. Moskophidis D. Mivechi N. J. Cell. Biochem. 2002; 86: 376-393Crossref PubMed Scopus (121) Google Scholar, 5Inouye S. Izu H. Takaki E. Suzuki H. Shirai M. Yokota Y. Ichikawa H. Fujimoto M. Nakai A. J. Biol. Chem. 2004; 279: 38701-38709Abstract Full Text Full Text PDF PubMed Scopus (89) Google Scholar). Gene expression analyses in various cell types, and organs derived from these Hsf1-/- mice revealed that HSF1 also regulates Hsp in physiological conditions (6Yan L.J. Christians E.S. Liu L. Xiao X. Sohal R.S. Benjamin I.J. EMBO J. 2002; 21: 5164-5172Crossref PubMed Scopus (191) Google Scholar, 7Zheng H. Li Z. J. Immunol. 2004; 173: 5929-5933Crossref PubMed Scopus (45) Google Scholar, 8Trinklein N.D. Murray J.I. Hartman S.J. Botstein D. Myers R.M. Mol. Biol. Cell. 2004; 15: 1254-1261Crossref PubMed Scopus (255) Google Scholar), providing accumulating evidence for the important function of HSF1 in maintaining cell homeostasis. Furthermore, those analyses and genome-wide screen demonstrated that numerous genes that were not classified as Hsps appeared to be HSF1-dependent (8Trinklein N.D. Murray J.I. Hartman S.J. Botstein D. Myers R.M. Mol. Biol. Cell. 2004; 15: 1254-1261Crossref PubMed Scopus (255) Google Scholar, 9Takaki E. Fujimoto M. Sugahara K. Nakahari T. Yonemura S. Tanaka Y. Hayashida N. Inouye S. Takemoto T. Yamashita H. Nakai A. J. Biol. Chem. 2006; 281: 4931-4937Abstract Full Text Full Text PDF PubMed Scopus (63) Google Scholar). Thus, HSF1 is clearly not restricted to the control of Hsp expression or the heat shock response. As shown by the complex phenotype of Hsf1 knock-out mice, HSF1 is involved in several specialized cell functions (e.g. placenta formation, immunity, placode development, cancer cell viability) (3Xiao X. Zuo X. Davis A.A. McMillan D.R. Curry B.B. Richardson J.A. Benjamin I.J. EMBO J. 1999; 18: 5943-5952Crossref PubMed Scopus (446) Google Scholar, 5Inouye S. Izu H. Takaki E. Suzuki H. Shirai M. Yokota Y. Ichikawa H. Fujimoto M. Nakai A. J. Biol. Chem. 2004; 279: 38701-38709Abstract Full Text Full Text PDF PubMed Scopus (89) Google Scholar, 10Fujimoto M. Izu H. Seki K. Fukuda K. Nishida T. Yamada S. Kato K. Yonemura S. Inouye S. Nakai A. EMBO J. 2004; 23: 4297-4306Crossref PubMed Scopus (187) Google Scholar, 11Dai C. Whitesell L. Rogers A.B. Lindquist S. Cell. 2007; 130: 1005-1018Abstract Full Text Full Text PDF PubMed Scopus (626) Google Scholar) and is essential for female reproduction (3Xiao X. Zuo X. Davis A.A. McMillan D.R. Curry B.B. Richardson J.A. Benjamin I.J. EMBO J. 1999; 18: 5943-5952Crossref PubMed Scopus (446) Google Scholar). We showed previously that Hsf1-/- female infertility is linked to the inability of Hsf1-/- oocytes to produce viable embryos after natural mating (12Christians E. Davis A.A. Thomas S.D. Benjamin I.J. Nature. 2000; 407: 693-694Crossref PubMed Scopus (228) Google Scholar). Nevertheless, the molecular and cellular mechanisms affected by the loss of HSF1 function in oocytes required further investigation to be better understood. Because HSF1 is highly expressed in oocytes, we hypothesized that it could regulate critical Hsps for the final development of oocytes into embryos. Although a series of studies separately analyzed several Hsps in rodent oocytes (see the references in Christians et al. (2Christians E.S. Benjamin I.J. Handb. Exp. Pharmacol. 2006; : 139-152Crossref PubMed Scopus (3) Google Scholar) and more recently for Hsp105, (13Vitale A.M. Calvert M.E. Mallavarapu M. Yurttas P. Perlin J. Herr J. Coonrod S. Mol. Reprod. Dev. 2007; 74: 608-616Crossref PubMed Scopus (74) Google Scholar)), no comprehensive picture of the expression and regulation of maternal Hsps emerged. Furthermore, Hsps are likely to be important maternal proteins because they act as chaperones, transiently interacting with other proteins (named clients for Hsp90 interacting candidates) to support numerous cellular processes ranging from cytoskeleton assembly to cell cycle control (14Kregel K.C. J. Appl. Physiol. 2002; 92: 2177-2186Crossref PubMed Scopus (1074) Google Scholar). However, the limited number of Hsp gene knockouts (Hsp25, Hsp70.1-Hsp70.3, Hsp90β) has not yet revealed the functional importance of any Hsp in oocytes either because there was no effect due to redundancy of Hsp function (15Huang L. Min J.N. Masters S. Mivechi N.F. Moskophidis D. Genesis. 2007; 45: 487-501Crossref PubMed Scopus (73) Google Scholar, 16Huang L. Mivechi N.F. Moskophidis D. Mol. Cell. Biol. 2001; 21: 8575-8591Crossref PubMed Scopus (117) Google Scholar, 17Hunt C.R. Dix D.J. Sharma G.G. Pandita R.K. Gupta A. Funk M. Pandita T.K. Mol. Cell. Biol. 2004; 24: 899-911Crossref PubMed Scopus (199) Google Scholar) or because the appearance of lethal phenotypes did not allow the appropriate analysis (e.g. Hsp90β knockouts died around 10 days post-coitus (18Voss A.K. Thomas T. Gruss P. Development. 2000; 127: 1-11Crossref PubMed Google Scholar)). Here we show that HSF1 differentially regulates Hsps and is required for the accumulation of large amounts of Hsp90α in fully grown oocytes. We provide evidence that both Hsp90-depleted (Hsf1-/-) and Hsp90-inhibited (17-(allylamino)-17-demethoxygelda-namycin (17AAG)-treated Hsf1+/+) oocytes suffer from a series of similar anomalies that impair meiosis progression, an obligatory step to prepare eggs for fertilization. This strongly suggests that Hsp90α deficit significantly contributes to the developmental defects seen in Hsf1-/- oocytes. Together, our data identify HSF1 as a new meiotic factor in mammals. Mice-Hsf1+/+ and Hsf1-/- mice, a gift from Dr. I. J. Benjamin (Salt Lake City, UT), have been described elsewhere (19McMillan D.R. Xiao X. Shao L. Graves K. Benjamin I.J. J. Biol. Chem. 1998; 273: 7523-7528Abstract Full Text Full Text PDF PubMed Scopus (431) Google Scholar). They were maintained in a mixed genetic background. Protocols for animal breeding and experiments were approved by the Departmental Veterinary Office (Haute-Garonne) according to French legislation. Oocyte Collection and Culture-Hsf1+/+ and Hsf1-/- oocytes were collected and cultured according to previously described procedures (20Van Cauwenberge A. Alexandre H. Int. J. Dev. Biol. 2000; 44: 409-420PubMed Google Scholar). Media (M2, M16, Sigma) were supplemented as indicated with IBMX (45 μg/ml, 1000× in DMSO, Sigma), 17AAG (1.78 μm, stock solution 1000× in DMSO, Sigma) (21de Carcer G. Cancer Res. 2004; 64: 5106-5112Crossref PubMed Scopus (57) Google Scholar), or cycloheximide (20 μg/ml, stock 2000× in ethanol). Real-time Reverse Transcription Quantitative PCR Analysis-Oocyte samples stored at -80 °C (20 oocytes) were thawed and mixed with up to 2 μl of lysis buffer (0.8% IGEPAL, (Sigma), 1 unit/μl RN as in, 5 mm dithiothreitol). Before reverse transcription, samples were heated at 75 °C for 5 min and transferred immediately to ice. DNase treatment was performed by adding 3 μl of DNA lysis buffer (2.5 mm MgCl2, 5× buffer (Invitrogen), 30 units of DNase I-RNase-free (Roche Applied Science) to the sample followed by incubation for 1 h at 25 °C and 5 m in at 70 °C. The reverse transcription reaction was carried out according to the manufacturer's instructions. The samples were subjected to oligonucleotide (dT)-primed first-strand cDNA synthesis in a final volume of 20 μl using the Super-ScriptII reverse transcriptase kit (Invitrogen). cDNA was synthesized at 42 °C for 1.5 h. The qPCR reaction was performed on an iCycler device (Bio-Rad) using Platinum SYBR Green qPCR Super-Mix-UDG (Invitrogen) according to the manufacturer's instructions. Primer sequences are listed in supplemental Table S1. Each reaction was performed in triplicate with an amount of cDNA corresponding to a single oocyte. Ribosomal protein S16 (S16) cDNA was used as an internal control to normalize the data, which were analyzed with the 2-ΔΔCT method (22Livak K.J. Schmittgen T.D. Methods. 2001; 25: 402-408Crossref PubMed Scopus (120954) Google Scholar). Chromatin Immunoprecipitation (ChIP)-The ChIP protocol was modified from Chang et al. (23Chang Y. Ostling P. Akerfelt M. Trouillet D. Rallu M. Gitton Y. El Fatimy R. Fardeau V. Le Crom S. Morange M. Sistonen L. Mezger V. Genes Dev. 2006; 20: 836-847Crossref PubMed Scopus (70) Google Scholar). Five ovaries were lysed in 3 ml of lysis buffer. Antibodies and primer sequences are listed in supplemental Tables S1 and S2. Western Blot Analysis-Fully grown oocytes stored at -80 °C were thawed, supplemented with sample buffer (24Laemmli U.K. Nature. 1970; 227: 680-685Crossref PubMed Scopus (206602) Google Scholar), and heated to 100 °C for 5 min, and total protein extracts were then subjected to one-dimensional SDS-PAGE followed by transfer on to nitrocellulose membranes. Blots were incubated in blocking buffer (Tris-buffered saline (TBS) containing 1% Tween 20 (TBS-T) and 5% milk) overnight at 4 °C and then incubated with the primary antibody in TBS containing 2-3% milk, 0.2% Tween 20) for 2 h at room temperature. Antibodies are listed in supplemental Table S2. The membranes were washed 3 times in TBS-T and then incubated in TBS-T, 2% milk to which appropriate horseradish peroxidase-conjugated secondary antibody was added. After several washes, membranes were developed with an enhanced chemiluminescence method (SuperSignal West Pico Chemiluminescent Substrate, Pierce). Immunostaining of Oocytes and Ovary Sections-Mouse oocytes were immunostained following the procedure described elsewhere (20Van Cauwenberge A. Alexandre H. Int. J. Dev. Biol. 2000; 44: 409-420PubMed Google Scholar) and analyzed with a Leica TCS SP-5 spectral confocal (Plateforme Toulouse RIO-Imaging, CBD-IFR109). For immunohistochemistry, mouse ovaries were fixed with Bouin, and histological preparations were performed according to a classical procedure (Plateau Technique d'Histopathologie Expérimentale de l'IFR30, Plateforme d'Exploration fonctionnelle/Génopole, Toulouse Midi-Pyrénées). Immunohistochemistry was performed according to a previously described procedure (25Salmand P.A. Jungas T. Fernandez M. Conter A. Christians E.S. Biol. Reprod. 2008; 79: 1092-1101Crossref PubMed Scopus (34) Google Scholar). Antibodies are described in supplemental Table S2. Imaging Analysis-A confocal microscope (Leica Microsystems, Heidelberg GmbH, Microscope confocal Leica SP5) was used for monitoring spindles and chromosomes in the immunolocalization experiments. An HCX PL APO 40.0×/1.25 NA oil immersion lens was used at room temperature. For fluorescein isothiocyanate, an argon laser was used with a 488-nm laser line and emission between 500- and 600-nm spectral detection range. The 543-nm laser line of a helium-neon laser provided excitation of Alexa Fluor 546, and fluorescence was collected using a 555-631-nm spectral detection range. For imaging TO-PRO-3, confocal images were obtained by exciting with the 633-nm laser line of a HeNe laser, and emission was collected through a 650-750-nm spectral detection range. For all confocal imaging experiments, a pinhole of 1 Airy unit was used. HSF1 Differentially Regulates Hsp Expression in Oocytes-Using reverse transcription followed by real-time PCR (qPCR), we examined mRNA levels of the major members of several Hsp families: Hsp25, Hsp60, Hsp70.1, Hsp70.3, Hsp90α, Hsp90β, Hsp105 (see gene descriptions in supplemental Table S1). These experiments revealed that Hsp90α transcripts were the most abundant in fully grown Hsf1+/+ oocytes. The levels of Hsp90β and Hsp105 transcripts were approximately one-fourth that of Hsp90α, whereas the transcripts of Hsp25, Hsp60, and Hsp70.1 were 100-fold less abundant, and Hsp70.3 transcripts were hardly detectable (Fig. 1A). Compared with Hsf1+/+, Hsf1-/- oocytes were markedly depleted in Hsp90α and exhibited visible down-regulation for Hsp70.1 and Hsp25 transcripts, but there was no difference for Hsp60 or Hsp90β transcripts (Fig. 1B). The effect of HSF1 deficiency on Hsp70.3 expression could not be determined because of the very low signals obtained in Hsf1+/+ and Hsf1-/- oocytes (Fig. 1, A and B). To demonstrate that HSF1 is the direct transcriptional regulator of Hsp90α gene, we undertook ChIP experiments using specific primers flanking HSF1 binding site (heat shock element (HSE)) located in Hsp90α promoter (Fig. 1C). We used total ovary extracts to obtain as much material as possible, as HSF1 was found to be specifically expressed in oocytes at all stages of ovarian oogenesis (supplemental Fig. S1). As shown in Fig. 1D, HSF1 bound the promoter of Hsp90α but not the regulatory region of Oct4, which is another gene that is highly active in oocytes. Taken together, these data indicate that HSF1 is required to store large amounts of Hsp90α transcripts. We further characterized the corresponding protein and compared the two cytoplasmic Hsp90s, Hsp90α and -β. Histological sections showed that Hsp90α was concentrated in oocyte cytoplasm and Hsp90β in follicular cells (Fig. 2A). Western blots performed with protein extracts from ovary revealed the presence of Hsp90α and -β (Fig. 2B). Hsp90α was easily detected in a total protein extract from 100 oocytes (Fig. 2B, after a 1-min exposure of the membrane). In contrast, even after a longer exposure (30 min), only a weak signal was visible in the case of Hsp90β (Fig. 2B). Thus, murine oocytes appear different from most somatic cells in that expression of Hsp90α overwhelmingly predominates over that of Hsp90β. In accordance with the reduction of Hsp90α transcripts, the level of Hsp90α protein is markedly reduced in Hsf1-/- oocytes (Fig. 2C). Disturbed Meiotic Progression in Hsf1-/- Oocytes-During development, oogonia enter meiosis at 13.5 days post-coitus, and oocytes remain blocked at prophase I until they are fully grown. Then, in response to hormonal signal or after experimental isolation from their ovarian follicles, oocytes resume meiosis, enter meiotic maturation, and progress to metaphase II (MII), at which stage they can be fertilized (Fig. 3A). Because fully grown Hsf1-/- oocytes do not exhibit morphological anomalies but are molecularly deficient in chaperones (this paper), we decided next to carefully examine these early developmental steps, which are essential prerequisites for obtaining normal embryos. We analyzed by video time-lapse microscopy the meiotic maturation of oocytes cultured in vitro. Resumption of meiosis, characterized by the disappearance of the nucleus (also named germinal vesicle (GV) breakdown (GVBD)), was seen to be significantly retarded in Hsf1-/- oocytes. The transition GV-GVBD occurred on average after 69.5 ± 8.65 min for Hsf1+/+ oocytes compared with 285 ± 26 min for Hsf1-/- oocytes (mean ± S.E. calculated from data presented in Fig. 3B, p < 0.001). Eventually, Hsf1-/- oocytes progressed through meiosis, but only 16.4% (n = 70/427) of Hsf1-/- oocytes reached MII (Fig. 3C), in comparison to 54.6% of Hsf1+/+ oocytes (n = 214/393). We retrospectively measured the duration of meiotic maturation in Hsf1-/- oocytes, which had reached the MII. Although they were all retarded for GVBD, they took the same time as Hsf1+/+ oocytes to progress from GVBD to MII (Fig. 3D). To better assess meiotic arrest in Hsf1-/- oocytes, we analyzed spindle morphology by immunostaining with anti-tubulin antibodies. Normally, the meiotic spindle progresses from a ball of microtubules to a bipolar structure (Figs. 3A and 4, A, I). At 14 h we observed two categories of Hsf1-/- oocytes (Fig. 4A, II and III, and supplemental Fig. S2). Representative examples of the first category are shown in Fig. 4A, II); these Hsf1-/- oocytes still exhibited a microtubular ball, indicating that they had failed to organize a bipolar spindle, and consequently, they did not achieve the first meiotic division. The second category corresponds to Hsf1-/- oocytes that had built a bipolar spindle (Fig. 4A, III) but which remained shorter and displayed a reduced microtubular density in comparison to Hsf1+/+ spindles (Fig. 4, B and C). Finally, oocyte maturation ends with the first meiotic division, resulting in the extrusion of the first polar body, which contains less than 20% of the oocyte volume. Hence, in contrast to most somatic cell divisions, meiotic cytokinesis is strongly asymmetrical. This characteristic was lost in a significant proportion of Hsf1-/- oocytes that had undergone the first meiotic division to produce an enlarged polar body or had even divided symmetrically (Fig. 4D and see Fig. 6A). From these data we conclude that meiosis in Hsf1-/- oocytes is severely affected, and we sought to test the hypothesis that this meiotic syndrome (GVBD delay, pro MI arrest, abnormal cytokinesis) is linked to the deficiency in Hsp90α expression we had identified. Timing of Meiotic Resumption (G2/M) Is under HSF1-Hsp90 Control-G2/M transition occurs spontaneously and rapidly after isolation of the oocytes from their ovarian follicles. To determine the role of HSF1-Hsp90 in this initial step of meiotic maturation, we compared Hsf1-/- with wild-type oocytes treated or not with 17AAG, a specific inhibitor of Hsp90 (26Whitesell L. Lindquist S.L. Nat. Rev. Cancer. 2005; 5: 761-772Crossref PubMed Scopus (1941) Google Scholar). Because the inhibitory action of 17AAG requires several hours, as shown in cancer cells (21de Carcer G. Cancer Res. 2004; 64: 5106-5112Crossref PubMed Scopus (57) Google Scholar), we preincubated fully grown oocytes for 12 h with the drug in IBMX medium to prevent resumption of meiosis. After removal of IBMX (t = 0 h), we scored GVBD at 2, 4, and 6 h (Fig. 5A). Within 2 h GVBD had occurred in 91% of untreated and in 3% of 17AAG-treated oocytes (Fig. 5B). At 6 h, about half of the 17AAG-treated oocytes had resumed meiosis, indicating they had been delayed for several hours in comparison to untreated oocytes. This delay was more severe than in Hsf1-/- oocytes probably due to the fact that the inhibitor abolished Hsp90 function completely, whereas HSF1 deficiency only reduced it. Because we observed the same delay in Hsf1-/- as in Hsf1+/+ oocytes when they were treated with 17AAG, we conclude that GVBD is dependent on Hsp90 function (Fig. 5B). In addition, we observed that treated Hsf1+/+ oocytes that had not undergone G2/M by 6 h could not resume meiosis and remained at the GV stage. This further suggests the importance of Hsp90 activity in meiosis resumption. GVBD or meiotic G2/M transition depends on a complex network of kinases and phosphatases that regulates maturation promoting factor (MPF) activity (Fig. 5C). Several kinases, such as PLK1, AKT, and CDK1, involved in the control of GVBD, are also Hsp90 clients, which means that these proteins transiently interact with Hsp90, thus becoming stabilized and acquiring their proper active conformation. Thus, in the absence of adequate Hsp90 activity, these proteins should be prone to degradation. We analyzed the levels of PLK1, AKT, and CDK1 by Western blots in both Hsf1-/- and 17AAG-treated Hsf1+/+ oocytes. PLK1 and CDK1 levels were clearly reduced, whereas the amount of AKT was unchanged (Fig. 5D). To further demonstrate that Hsp90 activity is important in preventing client degradation, we determined the stability of PLK1 and CDK1 in oocytes cultured as before with or without 17AAG and maintained under translation inhibition by cycloheximide for 6 and 12 h in culture. When we compared the amounts of PLK1 and CDK1 at these two time points, we could not detect significant changes for PLK1 (data not shown), but we observed that the CDK1 level was markedly reduced between 6 and 12 h of culture (Fig. 5E). Taken together, these data suggested that the GVBD is delayed both in Hsp90-depleted and Hsp90-inhibited oocytes because more time is required for accumulation of the amount of CDK1-cyclin B complex needed for maturation promoting factor activity to reach the threshold level necessary to reinitiate meiosis. Defective Asymmetrical Division in Maturing Oocytes Treated with 17AAG-To further test the effects of Hsp90 inhibition on meiosis progression and because long exposure to 17AAG partially prevented meiosis resumption, we collected and directly treated maturing oocytes. Under these conditions, the same percentage of MII was obtained in treated and nontreated oocytes. Nevertheless, we observed a significant number of cases of abnormal cytokinesis in 17AAG-treated oocytes, which produced larger polar bodies (77% for treated versus 4.5% for untreated Hsf1+/+ oocytes; Fig. 6A). This phenotype was strongly reminiscent of that we had noticed in 28% Hsf1-/- oocytes (Fig. 4D). Meiotic cytokinesis is normally delayed until the spindle has migrated to occupy a cortical position (see the diagram in Fig. 6B). One explanation of the formation of large polar bodies is that cytokinesis is deregulated and occurs too early before the spindle has normally reached the cortex. This was observed, for example, in oocytes deficient in MAD2, an important regulator of the spindle assembly checkpoint (27Homer H.A. McDougall A. Levasseur M. Yallop K. Murdoch A.P. Herbert M. Genes Dev. 2005; 19: 202-207Crossref PubMed Scopus (189) Google Scholar). However, this was not the case for Hsf1-/- or 17AAG-treated Hsf1+/+ oocytes, as the extrusion of the first polar body was not accelerated (Fig. 3D, supplemental Table S3). Thus, the defect could reside in the migration of the bipolar spindle itself in Hsf1-/- and 17AAG-treated oocytes. This was confirmed by the significantly lower frequency of spindles located near the cortex in the maturing oocytes (Fig. 6B). Reduced Activity of the MAP Kinase Pathway in Maturing Hsf1-/- Oocytes-At the molecular level, the MAP kinase (MAPK) pathway (Mos → MEK → ERK1/2) was shown to regulate the asymmetry of the first meiotic division. For example, genetic inactivation of Mos or depletion of MEK1 in mouse oocytes significantly increased the frequency of extrusion of a large polar body (28Choi T. Fukasawa K. Zhou R. Tessarollo L. Borror K. Resau J. Vande Woude G.F. Proc. Natl. Acad. Sci. U. S. A. 1996; 93: 7032-7035Crossref PubMed Scopus (192) Google Scholar, 29Yu L.Z. Xiong B. Gao W.X. Wang C.M. Zhong Z.S. Huo L.J. Wang Q. Hou Y. Liu K. Liu X.J. Schatten H. Chen D.Y. Sun Q.Y. Cell Cycle. 2007; 6: 330-338Crossref PubMed Scopus (70) Google Scholar). Therefore, we explored the hypothesis that reduced MAPK activity is the reason for the higher incidence of large polar bodies in oocytes lacking HSF1 and full activity of Hsp90. We consequently followed MAPK activity by immunodetection of the phosphorylated form of ERK1/2, the downstream target of MEK1. According to the literature, MAPK activity increases rapidly from 1 to 3 h post-GVBD and then remains stable until the end of maturation (30Verlhac M.H. Kubiak J.Z. Clarke H.J. Maro B. Development. 1994; 120: 1017-1025Crossref PubMed Google Scholar). Taking into account the observation that Hsf1-/- oocytes exhibit variable delays and block in meiosis progression, whereas 17AAG-treated oocytes are able to reach the MII stage, we first examined the level of ERK1/2-P by immunofluorescence (Fig. 7A). We selected the oocytes that exhibited a metaphase I plate and a bipolar spindle, indicating that they would probably undergo cytokinesis. Image analysis revealed that the relative amount of ERK1/2-P was lower in Hsf1-/- than in Hsf1+/+ oocytes (Fig. 7, B and C). Then we collected Hsf1-/- and 17AAG-treated oocytes after 14 h of culture and performed Western blots. Fig. 7D shows a representative example, indicating that the level of ERK1/2-P was decreased in those oocytes in comparison to Hsf1+/+ oocytes. Taken together, our morphological and molecular data indicate that Hsp90 activity is required to achieve normal, i.e. asymmetrical, oocyte meiosis I and suggest that this may occur through the regulation of the MAP kinase pathway. Mammalian oocytes are highly specialized cells engaged in a complex meiotic cell division, characterized by several "stops and starts" preceding the formation of the zygote through spermatozoon fusion and fertilization (Fig. 3A) (31Mehlmann L.M. Reproduction. 2005; 130: 791-799Crossref PubMed Scopus (336) Google Scholar). Once oocytes resume meiosis, they rely on maternal factors stored during oogenesis to sustain the subsequent developmental steps until the maternal-to-zygotic transition occurs (32Schultz R.M. Hum. Reprod. Update. 2002; 8: 323-331Crossref PubMed Scopus (368) Google Scholar, 33Hamatani T. Yamada M. Akutsu H. Kuji N. Mochimaru Y. Takano M. Toyoda M. Miyado K. Umezawa A. Yoshimura Y. Reproduction. 2008; 135: 581-592Crossref PubMed Scopus (32) Google Scholar). We previously reported that HSF1 is one of the few maternal factors in mammals required for female reproductive success (12Christians E. Davis A.A. Thomas S.D. Benjamin I.J. Nature. 2000; 407: 693-694Crossref PubMed Scopus (228) Google Scholar). In that paper we mainly focused our attention on post-mating events and concluded that Hsf1 loss of function prevented Hsf1-/- females from producing viable embryos, as they were all arrested before the blastocyst stage. To better understand such a maternal effect mutation from a developmental point of view, it is crucial to analyze molecular and cellular events carefully, starting with the oocyte itself. This was the purpose of the present study, and unexpectedly, we found that HSF1 plays a critical part in the regulation of oocyte meiosis and that this can be linked to its transcriptional regulation of Hsp90α, the prominent chaperone expressed in oocytes. From the evolutionary point of view, Hsp90 was previously shown to play a role in the meiotic maturation of Caenorhabditis elegans and Xenopus laevis oocytes, but no link was made with HSF1 in these studies (34Inoue T. Hirata K. Kuwana Y. Fujita M. Miwa J. Roy R. Yamaguchi Y. Dev. Growth Differ. 2006; 48: 25-32Crossref PubMed Scopus (33) Google Scholar, 35Fisher D.L. Mandart E. Doree M. EMBO J. 2000; 19: 1516-1524Crossref PubMed Scopus (57) Google Scholar). Furthermore, Hsp90 activity operated differently in the regulation of meiosis in these organisms (34Inoue T. Hirata K. Kuwana Y. Fujita M. Miwa J. Roy R. Yamaguchi Y. Dev. Growth Differ. 2006; 48: 25-32Crossref PubMed Scopus (33) Google Scholar, 35Fisher D.L. Mandart E. Doree M. EMBO J. 2000; 19: 1516-1524Crossref PubMed Scopus (57) Google Scholar). The nematode C. elegans uses the Daf-21/Hsp90 homolog to ensure the normal function of Wee (WEE-1.3), which is responsible for diakinesis arrest. Consequently, siRNA-mediated Daf-21 loss of function led to aberrant cell cycle progression and endomitotic oocytes (34Inoue T. Hirata K. Kuwana Y. Fujita M. Miwa J. Roy R. Yamaguchi Y. Dev. Growth Differ. 2006; 48: 25-32Crossref PubMed Scopus (33) Google Scholar). In lower vertebrates such as X. laevis, Hsp90 is instrumental in activating the Mos kinase that is essential to induce oocyte maturation in amphibians but not in mammals (35Fisher D.L. Mandart E. Doree M. EMBO J. 2000; 19: 1516-1524Crossref PubMed Scopus (57) Google Scholar). Taken together with these data, our results indicate that the involvement of Hsp90 in oocyte maturation is conserved through evolution, but the key Hsp90 clients appear to be different according to the species and to species-related regulation of oocyte maturation (36Han S.J. Conti M. Cell Cycle. 2006; 5: 227-231Crossref PubMed Scopus (132) Google Scholar). It is interesting to note that, whereas there is only one Hsp90 gene in lower species, mammals evolved with two cytoplasmic Hsp90 isoforms, Hsp90α and -β, both reported to be regulated by HSF1 (8Trinklein N.D. Murray J.I. Hartman S.J. Botstein D. Myers R.M. Mol. Biol. Cell. 2004; 15: 1254-1261Crossref PubMed Scopus (255) Google Scholar). Strikingly, oocytes contain almost exclusively the Hsp90α isoform and do not compensate with Hsp90β for Hsp90α down-regulation in the absence of HSF1. Although numerous studies did not distinguish between these two cytoplasmic Hsp90 isoforms, which are highly homologous, our data demonstrate that these two genes are independently regulated and acquire specialized functions in specific cell types (this paper and Voss et al. Ref. 18Voss A.K. Thomas T. Gruss P. Development. 2000; 127: 1-11Crossref PubMed Google Scholar). The meiotic syndrome described in the present paper (delayed G2/M transition, partial GVBD block, and defective asymmetrical division) has not been reported previously. With respect to the G2/M transition, CDK1, which was reported to be a critical limiting factor in female gametes (37Kanatsu-Shinohara M. Schultz R.M. Kopf G.S. Biol. Reprod. 2000; 63: 1610-1616Crossref PubMed Scopus (89) Google Scholar), was significantly diminished in Hsf1-/- and 17AAG-treated oocytes. Thus, our work appears to be in agreement with data collected from several cell lines in which Hsp90 inhibition was found to perturb G2/M transition and reduce CDK1 stability through increased proteasomal degradation (21de Carcer G. Cancer Res. 2004; 64: 5106-5112Crossref PubMed Scopus (57) Google Scholar, 38Garcia-Morales P. Carrasco-Garcia E. Ruiz-Rico P. Martinez-Mira R. Menendez-Gutierrez M.P. Ferragut J.A. Saceda M. Martinez-Lacaci I. 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Schultz R.M. Biol. Reprod. 2005; 72: 188-194Crossref PubMed Scopus (38) Google Scholar). So far there is no evidence of any link between these genes and Hsf1. In contrast, more is known about the role of Hsp90 and microtubule stabilization (21de Carcer G. Cancer Res. 2004; 64: 5106-5112Crossref PubMed Scopus (57) Google Scholar, 43Takaki E. Fujimoto M. Nakahari T. Yonemura S. Miyata Y. Hayashida N. Yamamoto K. Vallee R.B. Mikuriya T. Sugahara K. Yamashita H. Inouye S. Nakai A. J. Biol. Chem. 2007; 282: 37285-37292Abstract Full Text Full Text PDF PubMed Scopus (52) Google Scholar). Thus, deficient spindle organization could be because of severe disturbance of meiotic regulation in addition to defaults in microtubular assembly. Although more work is needed to understand this cellular anomaly better, it is likely to be responsible for meiotic arrest in Hsf1-/- oocytes. This leads to a dramatically small number of Hsf1-/- oocytes reaching the MII stage required for normal fertilization and development. The last, but significant, defect concerns the asymmetrical cytokinesis. It is important for oocytes to retain most of the maternal factors stored during oogenesis to sustain future embryonic development. Small polar bodies are extruded because before the division the meiotic spindle migrated from a central position to the cortex thanks to the actin cytoskeleton. Lack of spindle migration and formation of large polar bodies can be observed under several circumstances such as heat shock or brefeldin treatment, MAD2 depletion, and deficiency in the MAP kinase pathway (27Homer H.A. McDougall A. Levasseur M. Yallop K. Murdoch A.P. Herbert M. Genes Dev. 2005; 19: 202-207Crossref PubMed Scopus (189) Google Scholar, 28Choi T. Fukasawa K. Zhou R. Tessarollo L. Borror K. Resau J. Vande Woude G.F. Proc. Natl. Acad. Sci. U. S. 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We are currently working to identify and characterize plausible candidates. We are particularly grateful to C. Charry for genotyping Hsf1 knock-out mice. We thank A. Conter for immunohistochemistry and I. J. Benjamin, B. Ducommun, R. Morimoto, and our colleagues from the Centre de Biologie du Développement for generous gift of reagents and helpful discussion. We acknowledge the use of the imaging facilities (CBD-IFR109) and B. Ronsin for help with movie files. We are indebted to J. Smith for a critical review of the content and the English of the manuscript. Download .pdf (.33 MB) Help with pdf files