{"id":247,"date":"2017-10-24T09:22:20","date_gmt":"2017-10-24T13:22:20","guid":{"rendered":"https:\/\/health.uconn.edu\/cell-biology\/?page_id=247"},"modified":"2024-12-10T10:07:37","modified_gmt":"2024-12-10T15:07:37","slug":"lisa-mehlmann","status":"publish","type":"page","link":"https:\/\/health.uconn.edu\/cell-biology\/faculty-and-staff\/lisa-mehlmann\/","title":{"rendered":"Lisa Mehlmann"},"content":{"rendered":"

\"Lisa<\/a>Associate Professor
\nDepartment of Cell Biology<\/p>\n

Contact<\/h3>\n

Phone: 860-679-2703
\nEmail: lmehlman@uchc.edu<\/a>
\nOffice: E6052<\/p>\n

UConn Health
\n263 Farmington Avenue
\nFarmington, CT 06030<\/p>\n

Research Interests<\/h3>\n

Our lab is interested in elucidating cytoplasmic changes that occur in the mammalian oocyte that are important for the egg to become developmentally competent, as well as the mechanisms that cause these cytoplasmic changes to occur.\u00a0A complete understanding of these events will contribute to improving methods for maturing oocytes in vitro.<\/p>\n

Mammalian oocytes are stored within ovarian follicles at the prophase stage of meiosis.\u00a0They remain in prophase I as they and their associated follicles grow, and until a preovulatory surge of luteinizing hormone (LH) from the pituitary stimulates meiotic resumption to the metaphase II stage.\u00a0During the period of oocyte growth, meiotic arrest is maintained due to an insufficient amount of maturation-inducing proteins, in particular the cell cycle kinase CDK1.\u00a0However, as CDK1 accumulates in the oocyte, the oocyte becomes competent to mature and meiotic arrest shifts to a dependency on cAMP.\u00a0Work in my lab has established that the oocyte produces cAMP by the constitutive activity of the Gs-coupled receptor, GPR3 (Mehlmann et al., 2004).\u00a0GPR3 localizes in the plasma membrane and throughout the oocyte in early endosomes, and although it is constitutively active, its activity appears to be regulated via endocytosis\u00a0 (Lowther et al., 2011, 2013).\u00a0Oocytes lacking GPR3 are unable to maintain meiotic arrest\u00a0and resume meiosis spontaneously in the follicle, in the absence of an LH surge.\u00a0At the same time that the oocyte is producing cAMP, cAMP hydrolysis is prevented in the oocyte due to the inhibition of the phosphodiesterase, PDE3A, by follicle-derived cGMP (Norris et al., 2009).\u00a0High cGMP enters the oocyte through gap junctions and ensures that cAMP levels remain high until LH stimulates the follicle cells to reduce cGMP both in the follicle as well as the oocyte.\u00a0This in turn activates PDE3A in the oocyte to hydrolyze cAMP and cause meiotic resumption.\u00a0Available evidence indicates that similar mechanisms also function in human oocytes (DiLuigi et al., 2008).<\/p>\n

\"schematic
Stages of oocyte development.<\/strong>\u00a01) Oocytes express Gpr3 very early in development.\u00a0 GPR3 produces cAMP; the role of cAMP at early stages is unknown, but it might aid in the acquisition of meiotic competence.\u00a02)\u00a0As oocytes continue to grow, they accumulate CDK1 and other cell cycle proteins that allow them to become meiotically competent.\u00a03)\u00a0In response to LH, oocytes are stimulated to mature and undergo cytoplasmic changes that allow them become fertilizable and developmentally competent eggs (see below).<\/figcaption><\/figure>\n

Once LH stimulates the oocyte to mature, it undergoes numerous cytoplasmic changes during its transition to a fertilizable egg.\u00a0Many of these changes are not well understood.\u00a0However, it is well established that during maturation, the oocyte\u2019s endoplasmic reticulum (ER) undergoes a dramatic reorganization, such that the ER accumulates in the egg cortex (Mehlmann et al., 2005; Mann et al., 2010).\u00a0As the primary Ca2+<\/sup> storage organelle, the ER thereby becomes situated in the immediate region of the fertilizing sperm, which triggers Ca2+<\/sup> release through an IP3<\/sub>-mediated signaling cascade.\u00a0This release of Ca2+<\/sup> is critical for successful development of the newly-formed embryo.\u00a0Other changes that occur during oocyte maturation are an influx of Ca2+<\/sup> into the ER lumen, as well as a rearrangement of cortical granules to the cortex opposite the meiotic spindle.\u00a0In addition, the protein RGS2 becomes expressed during oocyte maturation to inhibit premature Ca2+<\/sup> release prior to fertilization (Bernhardt et al., 2015).\u00a0 The ability to release cortical granules at fertilization also develops during oocyte maturation.\u00a0 Cortical granule exocytosis is important for preventing polyspermy following fertilization.\u00a0 Our lab has been investigating mechanisms by which mature eggs exocytose cortical granules after fertilization.<\/p>\n

\"ER
Cytoplasmic changes during meiotic maturation in mouse oocytes.\u00a0<\/strong>Movement of endoplasmic reticulum (ER; red) to the egg cortex; increase in the number and change in localization of cortical granules (black dots), translation of RGS2, and an influx of Ca2+\u00a0(blue dots) into the ER lumen.<\/figcaption><\/figure>\n

 <\/p>\n

\"fluorescent
ER in a mature mouse egg, labelled with the lipophilic dye, DiI<\/strong>.\u00a0Notice the accumulation of ER in the cortex opposite the meiotic spindle (MS).<\/figcaption><\/figure>\n

Our lab is interested in elucidating cytoplasmic changes that occur in the oocyte that are important for the egg to become developmentally competent, as well as the mechanisms that cause these cytoplasmic changes to occur.\u00a0A complete understanding of these events will contribute to improving methods for maturing oocytes in vitro.<\/p>\n

Recent\u00a0 data:<\/strong><\/p>\n

Oocytes normally undergo the processes of endocytosis and exocytosis.\u00a0 In the immature oocyte, endocytosis appears to be associated with the regulation of meiosis, as preventing endocytosis causes the buildup of cAMP in the oocyte and blocks spontaneous meiotic resumption in oocytes that were isolated from follicles (Lowther et al., 2011).\u00a0 Using a newly developed method called Trim-away, we have shown that depleting the exocytotic SNARE protein, SNAP23, in follicle-enclosed oocytes causes them to undergo spontaneous maturation in the absence of LH (Mehlmann et al., 2019).\u00a0 This is attributed to the disconnection of the oocyte and the surrounding follicle cells, possibly due to the inability of the oocyte to place connexin 37 in the oocyte\u2019s plasma membrane.\u00a0 SNAP23 is also required for cortical granule exocytosis in the mature egg following fertilization.<\/p>\n

 <\/p>\n

\"Effects
Spontaneous meiotic resumption in the mouse oocyte when SNAP23 is depleted.<\/strong>\u00a0 A) Trim-away is effective in degrading endogenously expressed SNAP23 in follicle-enclosed oocytes.\u00a0 B) Oocytes undergo spontaneous meiotic resumption (GVBD) when SNAP23 is depleted in follicle-enclosed oocytes. C) Degradation of SNAP23 is associated with a disconnect between the oocyte and surrounding follicle cells.\u00a0 In this experiment, SNAP23 degradation was induced in follicle-enclosed oocytes and the continuity of gap junctions was determined by injecting a fluorescent dye into the oocyte.\u00a0 In the control follicle, the dye spreads readily from the oocyte to the granulosa cells.\u00a0 In the SNAP23-depleted oocyte, the dye does not diffuse out of the oocyte due to gap junction closure.<\/figcaption><\/figure>\n

 <\/p>\n

 <\/p>\n

\"fluorescent
SNAP23 is required for cortical granule exocytosis in the mouse egg.<\/strong>\u00a0 A) Cortical granules labelled with TRITC-LCA showing their distribution in untreated eggs, or in thimerosal-treated eggs.\u00a0 Cortical granules are absent in SNAP23-containing control eggs, whereas the cortical granules are retained in the cortex in the SNAP23-depleted eggs.\u00a0 B) ZP2 blot to evaluate cortical granule exocytosis.\u00a0 ZP2 is uncleaved in uninjected, untreated oocytes, but is cleaved in response in control eggs treated with thimerosal.\u00a0 ZP2 cannot be cleaved in SNAP23-depleted eggs. C) Thimerosal stimulates a series of repetitive Ca2+ oscillations in SNAP23-depleted eggs.<\/figcaption><\/figure>\n

New research on reproductive function in transgender males following testosterone therapy:<\/strong><\/p>\n

Recently, we have become interested in the quality of eggs retrieved from female mice that have been treated with testosterone.\u00a0 The rationale for the study is that transgender males (biologically female) often take high levels of testosterone to achieve desired male secondary sex characteristics such as lower voice and hair growth.\u00a0 Many transgender males wish to have biological children, but the effects of testosterone therapy on their eventual fertility is largely unknown.\u00a0 Current standard of care for transgender men who want to undergo egg retrieval is to first stop testosterone treatments and allow menses to resume; however, this treatment often triggers gender dysphoria in men and might cause them to avoid treatment, despite their desire for biological children.<\/p>\n

To test whether testosterone therapy needs to stop prior to obtaining eggs, we injected female mice with testosterone for 6 weeks.\u00a0 This treatment raised serum testosterone levels and had masculinizing effects such as clitoromegaly and caused the estrous cycle to stop.\u00a0 Ovaries from testosterone-treated mice weighed less than control ovaries but were histologically normal.\u00a0 Oocytes retrieved from testosterone-treated mice were meiotically competent and developed normal meiotic spindles after in vitro maturation.\u00a0 Importantly, testosterone-treated mice ovulated similar numbers of fertilizable eggs as controls in response to gonadotropin treatment.\u00a0 These experiments provide promising data that it might not be necessary for transgender men to be taken off of testosterone prior to gonadotropin treatment as the normal course of egg retrieval. \u00a0Full results may be obtained using the following link:\u00a0 https:\/\/www.biorxiv.org\/content\/10.1101\/2020.04.09.033803v1<\/a>.\u00a0 More work is being done to examine successful development of offspring following fertilization of eggs retrieved from testosterone-treated mice.<\/p>\n

\"Corpus
Sections from a control ovary (C) or a testosterone-treated ovary (T) from mice that were treated with eCG.<\/strong>\u00a0 Testosterone-treated ovaries are smaller than control ovaries and contain many fewer corpora lutea, indicated with asterisks.\u00a0 \u00a0Antral follicles are apparently normal, containing several layers of mural granulosa cells, intact cumulus cells, and oocytes with obvious nuclear envelopes.<\/figcaption><\/figure>\n
\"Graphs
Normal spindle development and fertilizability of oocytes retrieved from testosterone-treated mice.<\/strong>\u00a0 A) Testosterone treated mice (black bars) produce as many or more immature oocytes as controls.\u00a0 Unstimulated = immature oocytes obtained from ovaries of mice that have not undergone gonadotropin priming.\u00a0 eCG = immature oocytes obtained from the ovaries of eCG-stimulated mice.\u00a0 Ovulated = ovulated eggs retrieved after eCG and hCG injections.\u00a0 B) Normal spindle formation following in vitro maturation. C) Percentages of oocytes that cleaved following in vitro fertilization.<\/figcaption><\/figure>\n

Lab Members<\/a><\/p>\n

Selected Publications<\/h3>\n

Lisa M. Mehlmann, Tracy F. Uliasz, Siu-Pok Yee, Deborah Kaback, Katie M. Lowther. (2024) Generation and Characterization of a TRIM21 Overexpressing Mouse Line<\/a>. Genesis<\/em>; 62:e23616. https:\/\/doi.org\/10.1002\/dvg.23616.<\/p>\n

Prachi Godiwala, Tracy F. Uliasz, Katie M. Lowther, Deborah Kaback, and Lisa M. Mehlmann. (2023) Puberty Suppression Followed by Testosterone Therapy Does Not Impair Reproductive Potential in Female Mice<\/a>. Endocrinology<\/em>, 164, 1\u201310.<\/p>\n

Bartels CB, Uliasz TF, Lestz L, Mehlmann LM. (2021) Short term testosterone use in female mice does not impair fertilizability of eggs: Implications for the fertility care of transgender males<\/a>. Hum Reprod.<\/em>, 36: 189-198.<\/p>\n

Eisa AA, Bang S, Crawford KJ, Murphy EM, Feng WW, Dey S, Wells W, Kon N, Gu W, Mehlmann LM, Viyayaraghavan S, Kurokawa M.(2020) X-Linked\u00a0<\/span>Huwe1<\/em>\u00a0<\/span>Is Essential for Oocyte Maturation and Preimplantation Embryo Development<\/a>. iScience<\/em>., 23 (9):101523.<\/span><\/p>\n

Mehlmann, LM, Uliasz, TF, Lowther, KM. (2019) SNAP23 is required for constitutive and regulated exocytosis in mouse oocytes<\/a>. Biol of Reprod<\/em>., 101:338\u2013346.<\/p>\n

Firmani LD, Uliasz TF,\u00a0Mehlmann LM. 2018.\u00a0 The switch from cAMP-independent to cAMP-dependent arrest of meiotic prophase is associated with coordinated GPR3 and CDK1 expression in mouse oocytes<\/a>. Dev Biol<\/em>. 434:196-205.<\/p>\n

Bernhardt, M.L., Lowther, K.M., Padilla-Banks, E., McDonough, C.E., Lee, K.N., Evsikov, A.V., Uliasz, T.F., Chidiac, P., Williams, C.J., and<\/p>\n

Mehlmann, L.M. 2015. Regulator of G-protein signaling 2 (RGS2) suppresses premature calcium release in mouse eggs<\/a>. Development<\/em> 142: 2633-2640.<\/p>\n

Lowther, K.M. and Mehlmann, L.M. 2015. Embryonic Poly(A)-Binding Protein Is Required During Early Stages of Mouse Oocyte Development for Chromatin Organization, Transcriptional Silencing, and Meiotic
\nCompetence.<\/a>\u00a0Biol Reprod<\/em>. 93:43.<\/p>\n

Mehlmann, L.M.\u00a0 <\/strong>2013.\u00a0 Signalling for meiotic resumption in granulosa cells, cumulus cells, and oocyte.\u00a0 In:<\/em>\u00a0 <\/strong>Mammalian Oogenesis, <\/em>Coticchio, De Santis, and Albertini, eds. Springer Publishing Company, New York, NY, pp. 171-182.<\/p>\n

Lowther, K.M., Uliasz, T.F., Gotz, K.R., Nikolaev, V.O., and Mehlmann, L.M. 2013. Regulation of constitutive GPR3 signaling and surface localization by GRK2 and b-arrestin-2 overexpression in HEK293 cells<\/a>. PLoS One<\/em> 8: e65365.<\/p>\n

Mehlmann, L.M. 2013. Losing mom’s message: requirement for DCP1A and DCP2 in the degradation of maternal transcripts during oocyte maturation<\/a>. Biol Reprod. <\/em>88: 1-2.<\/p>\n

Guzeloglu-Kayisli, O., Lalioti, M.D., Aydiner, F., Sasson, I., Ilbay, O., Sakkas, D., Lowther, K.M., Mehlmann, L.M, and Seli, E. 2012. Embryonic poly(A)-binding protein (EPAB) is required for oocyte maturation and female fertility in mice<\/a>. Biochem J.<\/em> 446:47-58.<\/p>\n

Lowther, K.M., Nikolaev, V.O., and Mehlmann, L.M. 2011. Endocytosis in the mouse oocyte and its contribution to cAMP signaling during meiotic arrest<\/a>. Reproduction<\/em> 141:737-747.<\/p>\n

Mann, J.S., Lowther, K.M., and Mehlmann, L.M. 2010. Reorganization of the endoplasmic reticulum and development of Ca2+ release mechanisms during meiotic maturation of human oocytes<\/a>. Biol. Reprod.<\/em> 83:578\u2013583.<\/p>\n

Lowther, K.M., Weitzman, V.N., Maier, D., and Mehlmann, L.M. 2009. Maturation, fertilization, and the structure and function of the endoplasmic reticulum in cryopreserved mouse oocytes<\/a>. Biol. Reprod. <\/em>81:147-154.<\/p>\n

Norris, R.P., Ratzan, W.J., Freudzon, M., Mehlmann, L.M., Krall, J., Movsesian, M.A., Wang, H., Ke, H., Nikolaev, V.O., and Jaffe, L.A. 2009. Cyclic GMP from the surrounding somatic cells regulates cyclic AMP and meiosis in the mouse oocyte<\/a>. Development<\/em> 136:1869-1878.<\/p>\n

DiLuigi, A., Weitzman, V.N., Pace, M.C., Siano, L.J., Maier, D., and Mehlmann, L.M. 2008. Meiotic arrest in human oocytes is maintained by a Gs signaling pathway<\/a>. Biol. Reprod.<\/em> 78:667-672.<\/p>\n

Vaccari, S., Horner, K., Mehlmann, L.M., and Conti, M. 2008. Generation of mouse oocytes defective in cAMP synthesis and degradation: endogenous cyclic AMP is essential for meiotic arrest<\/a>. Dev. Biol. <\/em>316:124-134.<\/p>\n

Norris, R.P., Freudzon, M., Mehlmann, L.M., Cowan, A.E., Simon, A.M., Paul, D.L., Lampe, P.D., and Jaffe, L.A. 2008. Luteinizing hormone causes MAP kinase-dependent phosphorylation and closure of connexin 43 gap junctions in mouse ovarian follicles: one of two paths to meiotic resumption<\/a>. Development<\/em> 135:3229-3238.<\/p>\n

Norris, R.P., Freudzon, L., Freudzon, M., Hand, A.R., Mehlmann, L.M., and Jaffe, L.A. 2007. A Gs-linked receptor maintains meiotic arrest in mouse oocytes, but luteinizing hormone does not cause meiotic resumption by terminating receptor-Gs signaling<\/a>. Dev. Biol.<\/em> 310:240-249.<\/p>\n

Mehlmann, L.M., Kalinowski, R.R., Ross, L.F., Parlow, A.F., Hewlett, E.L. and Jaffe, L.A. 2006. Meiotic resumption in response to luteinizing hormone is independent of a Gi family G protein or calcium in the mouse oocyte<\/a>. Dev. Biol.<\/em> 299:345-355.<\/p>\n

Mehlmann, L.M. 2005. Stops and Starts in Mammalian Oocytes: Recent Advances in Understanding the Regulation of Meiotic Arrest and Oocyte Maturation<\/a>. Reproduction<\/em> 130:791-798.<\/p>\n

Freudzon, L., Norris, R.P., Hand, A.R., Tanaka, S., Saeki, Y., Jones, T.L.Z., Rasenick, M.M., Berlot, C.H., Mehlmann, L.M., and Jaffe, L.A. 2005. Regulation of meiotic prophase arrest in mouse oocytes by GPR3, a constitutive activator of the Gs G protein<\/a>. J. Cell Biol. <\/em>171:255-265.<\/p>\n

Mehlmann, L.M. 2005. Oocyte-specific expression of GPR3 is required for the maintenance of meiotic arrest in mouse oocytes<\/a>. Dev. Biol.<\/em> 288:397-404.<\/p>\n

Mehlmann, L.M., and Jaffe, L.A. 2005. SH2 domain-mediated activation of a SRC family kinase is not required to initiate Ca2+ release at fertilization in mouse eggs<\/a>. Reproduction<\/em>: 129: 557-564.<\/p>\n

Mehlmann, L.M., Saeki, Y., Tanaka, S., Brennan, T.J., Evsikov, A.V. Pendola, F.L., Knowles, B.B., Eppig, J.J., and Jaffe, L.A. 2004. The G s -linked receptor GPR3 maintains meiotic arrest in mammalian oocytes<\/a>. Science<\/em>: 306: 1947 – 1950.<\/p>\n

Kalinowski, R.R., Berlot, C.H., Jones, T.L.Z., Ross, L.F., Jaffe, L.A., and Mehlmann, L.M. 2004. Maintenance of meiotic prophase arrest in vertebrate oocytes by a G s protein-mediated pathway<\/a>. Dev. Biol.<\/em> 267: 1-13.<\/p>\n

Mehlmann, L.M., Jones, T.L.Z., and Jaffe, L.A. 2002. Meiotic arrest in the mouse follicle maintained by a G s protein in the oocyte<\/a>. Science<\/em> 297:1343-1345.<\/p>\n

Runft, L.L., Jaffe, L.A., and Mehlmann, L.M. 2002. Egg activation at fertilization: Where it all begins<\/a>. Dev. Biol.<\/em> 245:237-254.<\/p>\n","protected":false},"excerpt":{"rendered":"

Associate Professor Department of Cell Biology Contact Phone: 860-679-2703 Email: lmehlman@uchc.edu Office: E6052 UConn Health 263 Farmington Avenue Farmington, CT 06030 Research Interests Our lab is interested in elucidating cytoplasmic changes that occur in the mammalian oocyte that are important for the egg to become developmentally competent, as well as the mechanisms that cause these […]<\/p>\n","protected":false},"author":187,"featured_media":0,"parent":69,"menu_order":0,"comment_status":"closed","ping_status":"closed","template":"","meta":{"_acf_changed":false,"footnotes":""},"acf":[],"publishpress_future_action":{"enabled":false,"date":"2026-04-27 01:54:20","action":"change-status","newStatus":"draft","terms":[],"taxonomy":""},"_links":{"self":[{"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/pages\/247"}],"collection":[{"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/pages"}],"about":[{"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/types\/page"}],"author":[{"embeddable":true,"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/users\/187"}],"replies":[{"embeddable":true,"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/comments?post=247"}],"version-history":[{"count":65,"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/pages\/247\/revisions"}],"predecessor-version":[{"id":3588,"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/pages\/247\/revisions\/3588"}],"up":[{"embeddable":true,"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/pages\/69"}],"wp:attachment":[{"href":"https:\/\/health.uconn.edu\/cell-biology\/wp-json\/wp\/v2\/media?parent=247"}],"curies":[{"name":"wp","href":"https:\/\/api.w.org\/{rel}","templated":true}]}}