The primary aim of this project is to understand how gene regulation generates precise spatial patterns in embryonic development. A major focus of developmental biology is to characterize how networks of genes and their products create distinct and spatially separated cell types. However, the chemical reactions and transport processes underlying pattern formation are subject to numerous sources of variability and noise. Extrinsic sources include variability in temperature, size and maternally-supplied factors. Intrinsic noise arises from the low concentrations of many biological molecules and the random aspects of cell shape, orientation and movement. For development to reliably form complex body plans, gene network dynamics must be robust to these disruptive influences. Investigating the generation and control of spatial noise requires a quantitative methodology. Choosing one of the genetically best characterized model systems for embryonic patterning, anterior-posterior segmentation in the fruit fly Drosophila, allows us to simplify the biological challenges, so that we can focus on noise characterization. Our ultimate goal, however, is to contribute to the understanding, and perhaps limiting, of human birth defects. Our work should also be directly relevant to the variable disease outcomes associated with incomplete gene penetrance and to error control mechanisms for limiting cancer. Since studies of noise and variability require careful quantitation, a major focus of our work is the development of robust image processing and statistical techniques for separating signal from different types of noise in whole embryo images. Variability between signals from different embryos provides data on the variability of global parameters;the different types of intrinsic noise provide data on within-embryo variation. We use modeling to understand how variability or noise arises in the segmentation gene network, and how they might be controlled. We model dynamics at the promoter level (using DNA structure) and at the network level (with simplified gene-gene interactions). At the fine-scale promoter level, fitting stochastic models to normal and experimentally perturbed expression data reveals the degree to which noise is generated in gene expression, as well as revealing noise-reducing mechanisms. Network level modeling of between-embryo variability data (normal and experimentally perturbed) allows us to test hypotheses on what interactions make segmentation patterns robust. Mathematical analysis is used to characterize the dynamics of these processes. We have 2 specific aims in characterizing the transition from maternal to zygotic control of noise and variability in segmentation: 1) Maternal gradient formation: we will focus on unanswered questions regarding the temporal and sub-cellular patterning of bicoid mRNA and protein. 2) Zygotic gene interactions: we will focus on how gap and pair-rule genes buffer against maternal noise and variability and increase spatial precision as segments are specified. .

Public Health Relevance

Our project is aimed at understanding how genes interact in developing embryos to limit the effects of environmental and internal variability, so that tissues, organs and other parts of the body reliably form in the correct positions. Such gene regulation is also likely to be highly relevant to variable disease outcomes due to incomplete gene penetrance, and to error control mechanisms in cancer defense.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM072022-06A2
Application #
8184465
Study Section
Modeling and Analysis of Biological Systems Study Section (MABS)
Program Officer
Haynes, Susan R
Project Start
2004-04-01
Project End
2015-06-30
Budget Start
2011-09-19
Budget End
2012-06-30
Support Year
6
Fiscal Year
2011
Total Cost
$316,300
Indirect Cost
Name
State University New York Stony Brook
Department
Biostatistics & Other Math Sci
Type
Schools of Engineering
DUNS #
804878247
City
Stony Brook
State
NY
Country
United States
Zip Code
11794
Spirov, Alexander V; Myasnikova, Ekaterina M; Holloway, David M (2016) Sequential construction of a model for modular gene expression control, applied to spatial patterning of the Drosophila gene hunchback. J Bioinform Comput Biol 14:1641005
Shlemov, Alex; Golyandina, Nina; Holloway, David et al. (2015) Shaped 3D singular spectrum analysis for quantifying gene expression, with application to the early zebrafish embryo. Biomed Res Int 2015:986436
Zamdborg, Leonid; Holloway, David M; Merelo, Juan J et al. (2015) Forced evolution in silico by artificial transposons and their genetic operators: The ant navigation problem. Inf Sci (N Y) 306:88-110
Shlemov, Alex; Golyandina, Nina; Holloway, David et al. (2015) Shaped singular spectrum analysis for quantifying gene expression, with application to the early Drosophila embryo. Biomed Res Int 2015:689745
Holloway, David M; Spirov, Alexander V (2015) Mid-embryo patterning and precision in Drosophila segmentation: Krüppel dual regulation of hunchback. PLoS One 10:e0118450
Spirov, A V; Zagriychuk, E A; Holloway, D M (2014) Evolutionary Design of Gene Networks: Forced Evolution by Genomic Parasites. Parallel Process Lett 24:
Zagrijchuk, Elizaveta A; Sabirov, Marat A; Holloway, David M et al. (2014) In silico evolution of the hunchback gene indicates redundancy in cis-regulatory organization and spatial gene expression. J Bioinform Comput Biol 12:1441009
Spirov, Alexander; Holloway, David (2013) Using evolutionary computations to understand the design and evolution of gene and cell regulatory networks. Methods 62:39-55
Spirov, Alexander V; Holloway, David M (2013) Modeling the evolution of gene regulatory networks for spatial patterning in embryo development. Procedia Comput Sci 18:
Lopes, Francisco J P; Spirov, Alexander V; Bisch, Paulo M (2012) The role of Bicoid cooperative binding in the patterning of sharp borders in Drosophila melanogaster. Dev Biol 370:165-72

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