Abstract

The earliest developmental events occur while the zygotic genome is inactivated; thus, vertebrate development depends on maternally supplied gene products. Mutations that disrupt the genes that encode these necessary maternal factors, maternal-effect genes, can be teratogenic or lethal. Females with dysfunctional maternal-effect genes are grossly normal, due to normal gene function supplied by their mother. However, the progeny of these females develop abnormally regardless of their genotype. Despite increasing awareness of the significant impact maternal products have on vertebrate development and health, only a few maternal-effect genes have been experimentally evaluated through genetic or by interference approaches. For those genes that have been examined, it is clear that inadequate maternal contribution results in early embryonic lethality, or in less severe cases, developmental abnormalities. Similar genetic defects in humans are expected to result in failed implantation or miscarriage before a woman knows she is pregnant. Ten to twenty percent of pregnancies that are diagnosed result in miscarriage; however, many pregnancies go undetected. When these are factored in, the actual percentage of pregnancies that end in miscarriage is estimated to be significantly higher affecting 40-50% of all pregnancies, according to The March of Dimes, The American College of Obstetricians and Gynecologists, The Mayo clinic, and the National Institutes on Child Health and Development. Our long-term research goal is to determine the genetic pathways and cell biological events that direct development of the first axis of the vertebrate embryo. We will continue to use a combination of genetic, molecular genetics, cell biological, and affinity purification approaches in the zebrafish model system. In humans, losses of function mutations in genes whose products are essential for specification of the first embryonic axis will likely cause miscarriage due to severe developmental abnormalities. Moreover, the aspects of oocyte development that we study occur during fetal development in mammals; so, this process is not accessible in humans. In model systems such as zebrafish where fertilization and development of the embryo occur externally every egg produced can be examined for developmental abnormalities. Thus, the zebrafish is a powerful vertebrate system to study maternally controlled processes that are difficult to access in mammals and not possible to study in humans. Significantly, many of the genes known to regulate germline development are conserved from invertebrates to mammals; therefore, an improved understanding of the essential maternal genes that regulate the earliest patterning events of the germline and embryonic development in zebrafish will provide insight into the basis of birth defects, miscarriage, and infertility, and will facilitate comparison with human proteins.

Public Health Relevance

Primary oocytes of all animals including mammals, share conserved asymmetries including an ancient asymmetric structure in early oocytes known as the Balbiani body. We are using the zebrafish to understand the genes that instruct development of this conserved structure to determine its developmental function. Our work focuses on evolutionarily conserved RNA binding proteins and a vertebrate specific gene that produces a protein called Bucky ball. Bucky ball regulates cell polarity in oocytes, eggs, and embryos through an unknown pathway and mechanism. An improved understanding of this process may facilitate development of diagnostic tools to assess egg and embryo quality in assisted reproductive therapies.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM089979-06A1
Application #
9025623
Study Section
Development - 2 Study Section (DEV2)
Program Officer
Hoodbhoy, Tanya
Project Start
2009-12-01
Project End
2019-08-31
Budget Start
2015-09-22
Budget End
2016-08-31
Support Year
6
Fiscal Year
2015
Total Cost
$354,633
Indirect Cost
$142,278

  Institution

Name
Albert Einstein College of Medicine
Department
Type
DUNS #
079783367
City
Bronx
State
NY
Country
United States
Zip Code
10461

  Publications

Kaufman, Odelya H; Lee, KathyAnn; Martin, Manon et al. (2018) rbpms2 functions in Balbiani body architecture and ovary fate. PLoS Genet 14:e1007489
Forbes, Meredyth M; Draper, Bruce W; Marlow, Florence L (2017) Retraction: The polarity factor Bucky ball associates with the centrosome and promotes microtubule rearrangements to establish the oocyte axis in zebrafish. Development 144:1362
Santos-Ledo, Adrian; Garcia-Macia, Marina; Campbell, Philip D et al. (2017) Correction: Kinesin-1 promotes chondrocyte maintenance during skeletal morphogenesis. PLoS Genet 13:e1007099
Santos-Ledo, Adrian; Garcia-Macia, Marina; Campbell, Philip D et al. (2017) Kinesin-1 promotes chondrocyte maintenance during skeletal morphogenesis. PLoS Genet 13:e1006918
Marlow, Florence L (2017) Mitochondrial matters: Mitochondrial bottlenecks, self-assembling structures, and entrapment in the female germline. Stem Cell Res 21:178-186
Li-Villarreal, Nanbing; Forbes, Meredyth M; Loza, Andrew J et al. (2016) Dachsous1b cadherin regulates actin and microtubule cytoskeleton during early zebrafish embryogenesis. Development 143:1832
Kaufman, O H; Marlow, F L (2016) Methods to study maternal regulation of germ cell specification in zebrafish. Methods Cell Biol 134:1-32
Li-Villarreal, Nanbing; Forbes, Meredyth M; Loza, Andrew J et al. (2015) Dachsous1b cadherin regulates actin and microtubule cytoskeleton during early zebrafish embryogenesis. Development 142:2704-18
Campbell, Philip D; Heim, Amanda E; Smith, Mordechai Z et al. (2015) Kinesin-1 interacts with Bucky ball to form germ cells and is required to pattern the zebrafish body axis. Development 142:2996-3008
Marlow, Florence (2015) Primordial Germ Cell Specification and Migration. F1000Res 4:

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