Abstract

In sexually reproducing species, gametes are the only cells in the body that can give rise to a genetically complete new organism. In this sense, """"""""gametes are the stem cells of the species"""""""" (Wylie, 1999). Gametes originate from a small population of cells called primordial germ cells (PGCs) that form early in development. These unique cells retain full totipotency while somatic cells become progressively restricted in their fates. Eventually, PGCs migrate from their site of origin to the somatic gonads where they divide, enter meiosis and sexually differentiate. In Xenopus, it is thought that PGCs are determined by inheritance of germ plasm, a specialized cytoplasmic domain containing unique RNAs and proteins. Virtually nothing is known about how PGCs preserve their totipotency or what functions germ plasm components play in POC development. Several germ plasm specific RNAs have been isolated, including Xdazl a member of the DAZ family in humans (King et al., 1999). We found that maternal depletion of Xdazl results in the severe reduction or loss of PGCs because they fail to migrate out of the endoderm (Houston and King, 2000). Xcat-2, DEADSouth, and Xpat are other germ plasm specific RNAs that have been characterized, but whose functions are not known. In this proposal, experiments are outlined to explore how germ cell fate is determined and will address the following questions: I. What mechanism permits PGCs to retain a totipotent fate while surrounding cells in the vegetal mass become committed to an endoderm fate? What role, if any, does endoderm play in this process? II. What steps in PGC development require the germ plasm components Xcat-2, DEADSouth, Xdazl, and Xpat? What specific molecular functions do Xdazl and DEADSouth proteins perform? III. What is the mechanism of translational repression of the germ plasm RNAs Xdazl, Xcat2, and DEADSouth during oogenesis? A method for targeting green fluorescent protein (GFP) expression to the germ plasm is presented that will allow PGCs to be followed or isolated at different times in development. This procedure will make PGCs accessible to biochemical and molecular studies for the first time. Immunocytochemistry and in situ hybridization will be used to determine when PGCs become transcriptionally active and whether they express genes diagnostic for endoderm. Gain-of-function, loss-of-function, and over-expression experiments targeting the germ plasm RNAs will pinpoint the steps that require these genes. Oocyte injections of deletion mutants in the UTR regions of Xcat2 and Xdazl will reveal cis-acting elements required for translational repression. These cis elements will be used to affinity purify trans-acting factors. Results from these proposed studies will offer significant insights into how the germline forms in Xenopus and in general as key aspects of PGC development (totipotency, migration) are likely conserved across phyla.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM033932-16A1
Application #
6331219
Study Section
Cell Development and Function Integrated Review Group (CDF)
Program Officer
Zatz, Marion M
Project Start
1988-08-01
Project End
2005-03-31
Budget Start
2001-04-01
Budget End
2002-03-31
Support Year
16
Fiscal Year
2001
Total Cost
$344,207
Indirect Cost

  Institution

Name
University of Miami School of Medicine
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
City
Miami
State
FL
Country
United States
Zip Code
33146

  Publications

Mei, Wenyan; Jin, Zhigang; Lai, Fangfang et al. (2013) Maternal Dead-End1 is required for vegetal cortical microtubule assembly during Xenopus axis specification. Development 140:2334-44
Lai, Fangfang; Singh, Amar; King, Mary Lou (2012) Xenopus Nanos1 is required to prevent endoderm gene expression and apoptosis in primordial germ cells. Development 139:1476-86
Luo, Xueting; Nerlick, Steve; An, Weijun et al. (2011) Xenopus germline nanos1 is translationally repressed by a novel structure-based mechanism. Development 138:589-98
Lai, Fangfang; Zhou, Yi; Luo, Xueting et al. (2011) Nanos1 functions as a translational repressor in the Xenopus germline. Mech Dev 128:153-63
Venkatarama, Thiagarajan; Lai, Fangfang; Luo, Xueting et al. (2010) Repression of zygotic gene expression in the Xenopus germline. Development 137:651-60
Rodrigues, Claudia O; Nerlick, Steve T; White, Elsie L et al. (2008) A Myc-Slug (Snail2)/Twist regulatory circuit directs vascular development. Development 135:1903-11
Song, Hye-Won; Cauffman, Karen; Chan, Agnes P et al. (2007) Hermes RNA-binding protein targets RNAs-encoding proteins involved in meiotic maturation, early cleavage, and germline development. Differentiation 75:519-28
Lewis, Raymond A; Mowry, Kimberly L (2007) Ribonucleoprotein remodeling during RNA localization. Differentiation 75:507-18
King, Mary Lou; Messitt, Timothy J; Mowry, Kimberly L (2005) Putting RNAs in the right place at the right time: RNA localization in the frog oocyte. Biol Cell 97:19-33
Machado, Rachel J; Moore, Wendy; Hames, Richard et al. (2005) Xenopus Xpat protein is a major component of germ plasm and may function in its organisation and positioning. Dev Biol 287:289-300

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