Activity
Time:
M.S. Defense: Natasha Pavlovikj
Date:
12:00 pm –
1:00 pm
Zoom
M.S. Defense: Natasha Pavlovikj
Monday, February 28, 2022
Noon
Zoom: https://unl.zoom.us/j/95990415134
Meeting ID: 959 9041 5134
“Comparative Analysis Of De Novo Transcriptome Assembly Pipelines For Diploid Wheat”
Gene expression and transcriptome analysis are currently one of the main focuses of research for a great number of scientists. However, the assembly of raw sequence data to obtain a draft transcriptome of an organism is a complex multi-stage process usually composed of pre-processing, assembling, and post-processing. Each of these stages includes multiple steps such as data cleaning, error correction and assembly validation. Different combinations of steps, as well as different computational methods for the same step, generate transcriptome assemblies with different accuracy. Thus, using a combination that generates more accurate assemblies is crucial for any novel biological discoveries. Implementing accurate transcriptome assembly requires a great knowledge of different algorithms, bioinformatics tools and software that can be used in an analysis pipeline. Many pipelines can be represented as automated scalable scientific workflows that can be run simultaneously on powerful distributed and computational resources, such as Campus Clusters, Grids, and Clouds, and speed-up the analyses. In this thesis, we 1) compared and optimized de novo transcriptome assembly pipelines for diploid wheat; 2) investigated the impact of a few key parameters for generating accurate transcriptome assemblies, such as digital normalization and error correction methods, de novo assemblers and k-mer length strategies; 3) built distributed and scalable scientific workflow for blast2cap3, a step from the transcriptome assembly pipeline for protein-guided assembly, using the Pegasus Workflow Management System (WMS); and 4) deployed and examined the scientific workflow for blast2cap3 on two different computational platforms. Based on the analysis performed in this paper, we conclude that the best transcriptome assembly is produced when the error correction method is used with Velvet Oases and the “multi-k” strategy. Moreover, the performed experiments show that the Pegasus WMS implementation of blast2cap3 reduces the running time for more than 95% compared to its current serial implementation. The results presented in this thesis provide valuable insight for designing good de novo transcriptome assembly pipeline and show the importance of using scientific workflows for executing computationally demanding pipelines.
Committee members:
Dr. Jitender S. Deogun (advisor)
Dr. Etsuko Moriyama
Dr. Hongfeng Yu
Monday, February 28, 2022
Noon
Zoom: https://unl.zoom.us/j/95990415134
Meeting ID: 959 9041 5134
“Comparative Analysis Of De Novo Transcriptome Assembly Pipelines For Diploid Wheat”
Gene expression and transcriptome analysis are currently one of the main focuses of research for a great number of scientists. However, the assembly of raw sequence data to obtain a draft transcriptome of an organism is a complex multi-stage process usually composed of pre-processing, assembling, and post-processing. Each of these stages includes multiple steps such as data cleaning, error correction and assembly validation. Different combinations of steps, as well as different computational methods for the same step, generate transcriptome assemblies with different accuracy. Thus, using a combination that generates more accurate assemblies is crucial for any novel biological discoveries. Implementing accurate transcriptome assembly requires a great knowledge of different algorithms, bioinformatics tools and software that can be used in an analysis pipeline. Many pipelines can be represented as automated scalable scientific workflows that can be run simultaneously on powerful distributed and computational resources, such as Campus Clusters, Grids, and Clouds, and speed-up the analyses. In this thesis, we 1) compared and optimized de novo transcriptome assembly pipelines for diploid wheat; 2) investigated the impact of a few key parameters for generating accurate transcriptome assemblies, such as digital normalization and error correction methods, de novo assemblers and k-mer length strategies; 3) built distributed and scalable scientific workflow for blast2cap3, a step from the transcriptome assembly pipeline for protein-guided assembly, using the Pegasus Workflow Management System (WMS); and 4) deployed and examined the scientific workflow for blast2cap3 on two different computational platforms. Based on the analysis performed in this paper, we conclude that the best transcriptome assembly is produced when the error correction method is used with Velvet Oases and the “multi-k” strategy. Moreover, the performed experiments show that the Pegasus WMS implementation of blast2cap3 reduces the running time for more than 95% compared to its current serial implementation. The results presented in this thesis provide valuable insight for designing good de novo transcriptome assembly pipeline and show the importance of using scientific workflows for executing computationally demanding pipelines.
Committee members:
Dr. Jitender S. Deogun (advisor)
Dr. Etsuko Moriyama
Dr. Hongfeng Yu