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GRIM-Filter: Fast Seed Location Filtering in DNA Read Mapping Using Processing-in-Memory Technologies

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 نشر من قبل Jeremie Kim
 تاريخ النشر 2017
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Motivation: Seed location filtering is critical in DNA read mapping, a process where billions of DNA fragments (reads) sampled from a donor are mapped onto a reference genome to identify genomic variants of the donor. State-of-the-art read mappers 1) quickly generate possible mapping locations for seeds (i.e., smaller segments) within each read, 2) extract reference sequences at each of the mapping locations, and 3) check similarity between each read and its associated reference sequences with a computationally-expensive algorithm (i.e., sequence alignment) to determine the origin of the read. A seed location filter comes into play before alignment, discarding seed locations that alignment would deem a poor match. The ideal seed location filter would discard all poor match locations prior to alignment such that there is no wasted computation on unnecessary alignments. Results: We propose a novel seed location filtering algorithm, GRIM-Filter, optimized to exploit 3D-stacked memory systems that integrate computation within a logic layer stacked under memory layers, to perform processing-in-memory (PIM). GRIM-Filter quickly filters seed locations by 1) introducing a new representation of coarse-grained segments of the reference genome, and 2) using massively-parallel in-memory operations to identify read presence within each coarse-grained segment. Our evaluations show that for a sequence alignment error tolerance of 0.05, GRIM-Filter 1) reduces the false negative rate of filtering by 5.59x--6.41x, and 2) provides an end-to-end read mapper speedup of 1.81x--3.65x, compared to a state-of-the-art read mapper employing the best previous seed location filtering algorithm. Availability: The code is available online at: https://github.com/CMU-SAFARI/GRIM



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Motivation: Seed filtering is critical in DNA read mapping, a process where billions of DNA fragments (reads) sampled from a donor are mapped onto a reference genome to identify genomic variants of the donor. Read mappers 1) quickly generate possible mapping locations (i.e., seeds) for each read, 2) extract reference sequences at each of the mapping locations, and then 3) check similarity between each read and its associated reference sequences with a computationally expensive dynamic programming algorithm (alignment) to determine the origin of the read. Location filters come into play before alignment, discarding seed locations that alignment would have deemed a poor match. The ideal location filter would discard all poor matching locations prior to alignment such that there is no wasted computation on poor alignments. Results: We propose a novel filtering algorithm, GRIM-Filter, optimized to exploit emerging 3D-stacked memory systems that integrate computation within a stacked logic layer, enabling processing-in-memory (PIM). GRIM-Filter quickly filters locations by 1) introducing a new representation of coarse-grained segments of the reference genome and 2) using massively-parallel in-memory operations to identify read presence within each coarse-grained segment. Our evaluations show that for 5% error acceptance rates, GRIM-Filter eliminates 5.59x-6.41x more false negatives and exhibits end-to-end speedups of 1.81x-3.65x compared to mappers employing the best previous filtering algorithm.
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