sequencing platform Search Results


minion sequencing instrument  (Oxford Nanopore)
96
Oxford Nanopore minion sequencing instrument
Minion Sequencing Instrument, supplied by Oxford Nanopore, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/minion sequencing instrument/product/Oxford Nanopore
Average 96 stars, based on 1 article reviews
minion sequencing instrument - by Bioz Stars, 2026-06
96/100 stars
  Buy from Supplier
flongle sequencing expansion  (Oxford Nanopore)
93
Oxford Nanopore flongle sequencing expansion
Flongle Sequencing Expansion, supplied by Oxford Nanopore, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/flongle sequencing expansion/product/Oxford Nanopore
Average 93 stars, based on 1 article reviews
flongle sequencing expansion - by Bioz Stars, 2026-06
93/100 stars
  Buy from Supplier
sequencing platforms  (10X Genomics)
86
10X Genomics sequencing platforms
A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome <t>sequencing</t> (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).
Sequencing Platforms, supplied by 10X Genomics, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/sequencing platforms/product/10X Genomics
Average 86 stars, based on 1 article reviews
sequencing platforms - by Bioz Stars, 2026-06
86/100 stars
  Buy from Supplier
next-generation sequencing (ngs) platform panel comprised genes frequently mutated in myeloid neoplasms raindance thunderbolts myeloid panel  (RainDance Technologies)
90
RainDance Technologies next-generation sequencing (ngs) platform panel comprised genes frequently mutated in myeloid neoplasms raindance thunderbolts myeloid panel
A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome <t>sequencing</t> (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).
Next Generation Sequencing (Ngs) Platform Panel Comprised Genes Frequently Mutated In Myeloid Neoplasms Raindance Thunderbolts Myeloid Panel, supplied by RainDance Technologies, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/next-generation sequencing (ngs) platform panel comprised genes frequently mutated in myeloid neoplasms raindance thunderbolts myeloid panel/product/RainDance Technologies
Average 90 stars, based on 1 article reviews
next-generation sequencing (ngs) platform panel comprised genes frequently mutated in myeloid neoplasms raindance thunderbolts myeloid panel - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
nova6000 sequencing platform  (MyGenostics Inc)
90
MyGenostics Inc nova6000 sequencing platform
A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome <t>sequencing</t> (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).
Nova6000 Sequencing Platform, supplied by MyGenostics Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/nova6000 sequencing platform/product/MyGenostics Inc
Average 90 stars, based on 1 article reviews
nova6000 sequencing platform - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
dna sequencing platform  (Tempus Labs Inc)
90
Tempus Labs Inc dna sequencing platform
A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome <t>sequencing</t> (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).
Dna Sequencing Platform, supplied by Tempus Labs Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/dna sequencing platform/product/Tempus Labs Inc
Average 90 stars, based on 1 article reviews
dna sequencing platform - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
sequencing, variant calling and annotation platform  (Knome Inc)
90
Knome Inc sequencing, variant calling and annotation platform
A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome <t>sequencing</t> (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).
Sequencing, Variant Calling And Annotation Platform, supplied by Knome Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/sequencing, variant calling and annotation platform/product/Knome Inc
Average 90 stars, based on 1 article reviews
sequencing, variant calling and annotation platform - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
illumina 2000/2500 sequence platform  (LC Sciences)
90
LC Sciences illumina 2000/2500 sequence platform
A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome <t>sequencing</t> (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).
Illumina 2000/2500 Sequence Platform, supplied by LC Sciences, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/illumina 2000/2500 sequence platform/product/LC Sciences
Average 90 stars, based on 1 article reviews
illumina 2000/2500 sequence platform - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
targeted next generation sequencing  (Integragen sa)
90
Integragen sa targeted next generation sequencing
A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome <t>sequencing</t> (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).
Targeted Next Generation Sequencing, supplied by Integragen sa, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/targeted next generation sequencing/product/Integragen sa
Average 90 stars, based on 1 article reviews
targeted next generation sequencing - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
sequence-engineered mrna-lnp platform  (CureVac Inc)
90
CureVac Inc sequence-engineered mrna-lnp platform
RNA vaccines against influenza virus.*
Sequence Engineered Mrna Lnp Platform, supplied by CureVac Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/sequence-engineered mrna-lnp platform/product/CureVac Inc
Average 90 stars, based on 1 article reviews
sequence-engineered mrna-lnp platform - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
whole genome sequencing oxford nanopore gridion platform  (Oxford Nanopore)
90
Oxford Nanopore whole genome sequencing oxford nanopore gridion platform
RNA vaccines against influenza virus.*
Whole Genome Sequencing Oxford Nanopore Gridion Platform, supplied by Oxford Nanopore, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/whole genome sequencing oxford nanopore gridion platform/product/Oxford Nanopore
Average 90 stars, based on 1 article reviews
whole genome sequencing oxford nanopore gridion platform - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier
sequencing platforms  (Oxford Nanopore)
90
Oxford Nanopore sequencing platforms
RNA vaccines against influenza virus.*
Sequencing Platforms, supplied by Oxford Nanopore, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/sequencing platforms/product/Oxford Nanopore
Average 90 stars, based on 1 article reviews
sequencing platforms - by Bioz Stars, 2026-06
90/100 stars
  Buy from Supplier

Image Search Results


A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome sequencing (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Journal: PLoS ONE

Article Title: Protection of the C . elegans germ cell genome depends on diverse DNA repair pathways during normal proliferation

doi: 10.1371/journal.pone.0250291

Figure Lengend Snippet: A. L4 larvae (F1 generation) from a parental founder strain (P0) were individually picked onto NGM plates and allowed to self-fertilize prior to picking individual L4 larvae of the next generation (F2) from each F1 plate. This process was repeated until clonal lines reached generation F20 or F40. Clonal lines were then allowed to expand, harvested, and prepared for whole genome sequencing (Materials and Methods). B. Mutation types and their location on the 6 C . elegans chromosomes (I-V and X) across all wild-type samples and mutation classes. The height of the white bars corresponds to the length of the respective C . elegans chromosome. Single nucleotide variants are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D) and insertions (I) by a triangle, and structural variants (SVs) by a line. C. Average number of heterozygous mutations in the N2 wild-type genome per generation across all mutation classes and types. Single nucleotide variants are shown in the context of their 5’ and 3’ base. Grey bars denote 95% credible intervals for the number of mutations in each type. “Complex indels” class denotes deletions with insertions. Data for N2 was previously shown in ( Fig 1C) . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Article Snippet: In summary, DNA sequencing was performed using Illumina HiSeq 2000 and 10X Genomics short reads sequencing platforms at 100 bp paired-end, with a mean coverage of 50x.

Techniques: Sequencing, Mutagenesis

Mutation rates are shown as number of heterozygous mutations per generation for N2 wild-type (WT), and mutants used in this study grouped by the major DNA repair pathway they contribute to; direct damage reversal (DR), base excision repair (BER), nucleotide excision repair (NER), DNA double-strand break repair (DSBR), translesion synthesis (TLS), crosslink repair (ICLR), spindle assembly checkpoint (SAC), apoptosis, and mismatch repair (MMR). Base substitutions are shown in red (top), indels in green (center) and structural variants in blue (bottom). Dotted lines denote the mutation rates for wild-type. Error bars show the 95% confidence intervals; large dots represent variants with 2-fold increased or decreased mutation rates over N2 wild-type which are statistically significant with a false discovery rate (FDR) below 5%. All CIs which extend below the lower edge of the plot have zero as their lower border. Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Journal: PLoS ONE

Article Title: Protection of the C . elegans germ cell genome depends on diverse DNA repair pathways during normal proliferation

doi: 10.1371/journal.pone.0250291

Figure Lengend Snippet: Mutation rates are shown as number of heterozygous mutations per generation for N2 wild-type (WT), and mutants used in this study grouped by the major DNA repair pathway they contribute to; direct damage reversal (DR), base excision repair (BER), nucleotide excision repair (NER), DNA double-strand break repair (DSBR), translesion synthesis (TLS), crosslink repair (ICLR), spindle assembly checkpoint (SAC), apoptosis, and mismatch repair (MMR). Base substitutions are shown in red (top), indels in green (center) and structural variants in blue (bottom). Dotted lines denote the mutation rates for wild-type. Error bars show the 95% confidence intervals; large dots represent variants with 2-fold increased or decreased mutation rates over N2 wild-type which are statistically significant with a false discovery rate (FDR) below 5%. All CIs which extend below the lower edge of the plot have zero as their lower border. Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Article Snippet: In summary, DNA sequencing was performed using Illumina HiSeq 2000 and 10X Genomics short reads sequencing platforms at 100 bp paired-end, with a mean coverage of 50x.

Techniques: Mutagenesis, Translesion Synthesis, Sequencing

A. Mutational signatures of BER, NER, and DR mutants that display statistically significantly different mutation spectra than wild-type shown as the number of mutations per generation across all mutation classes. Underscores (bold coloured bars) below each mutation profile indicate mutation types where the total mutation numbers are different from wild-type, three stars indicate genotypes with significantly different rates of substitutions, indels or SVs compared to those in wild-type (FDR < 5%). Single nucleotide variants are shown in the context of their 5’ and 3’ base context. B. Number of mutations of all classes shown for each individual sequenced line of the indicated genotype and generation. The four sequenced wild-type P0 lines reflect the variance present in initial generations. Mutations are shown cumulatively with mutations present in generation F20 included in F40. C. Mutation types of all classes and their location on the 6 C . elegans chromosomes (I-V and X) observed across agt-2 mutant lines. The height of the white bars corresponds to the length of each individual chromosome. Single nucleotide variants (SNVs) are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D), insertions (I), and deletions with insertions (DI) by a triangle, and structural variants (SVs) by a line. Clustered mutations that are present within a single agt-2 line are depicted by enlarged bold symbols. An analysis of brca-1 , him-6 and smc-6 swas previously shown in . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Journal: PLoS ONE

Article Title: Protection of the C . elegans germ cell genome depends on diverse DNA repair pathways during normal proliferation

doi: 10.1371/journal.pone.0250291

Figure Lengend Snippet: A. Mutational signatures of BER, NER, and DR mutants that display statistically significantly different mutation spectra than wild-type shown as the number of mutations per generation across all mutation classes. Underscores (bold coloured bars) below each mutation profile indicate mutation types where the total mutation numbers are different from wild-type, three stars indicate genotypes with significantly different rates of substitutions, indels or SVs compared to those in wild-type (FDR < 5%). Single nucleotide variants are shown in the context of their 5’ and 3’ base context. B. Number of mutations of all classes shown for each individual sequenced line of the indicated genotype and generation. The four sequenced wild-type P0 lines reflect the variance present in initial generations. Mutations are shown cumulatively with mutations present in generation F20 included in F40. C. Mutation types of all classes and their location on the 6 C . elegans chromosomes (I-V and X) observed across agt-2 mutant lines. The height of the white bars corresponds to the length of each individual chromosome. Single nucleotide variants (SNVs) are indicated by a dot, dinucleotide variants (DNVs) by a square, indels divided in deletions (D), insertions (I), and deletions with insertions (DI) by a triangle, and structural variants (SVs) by a line. Clustered mutations that are present within a single agt-2 line are depicted by enlarged bold symbols. An analysis of brca-1 , him-6 and smc-6 swas previously shown in . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Article Snippet: In summary, DNA sequencing was performed using Illumina HiSeq 2000 and 10X Genomics short reads sequencing platforms at 100 bp paired-end, with a mean coverage of 50x.

Techniques: Mutagenesis, Sequencing

A. Mutational signatures of DSBR mutants that exhibited statistically significant different mutation rates to wild-type displayed in numbers of mutations per generation. Bold coloured bars denote individual mutation classes where the number of mutations is different from wild-type, an underscore below each mutation profile indicates mutation types with total mutation numbers different from wild-type, and three stars indicate genotypes which have rates of substitutions, indels or SVs significantly different compared to wild-type (FDR < 5%). B. Estimated composition of structural variants per generation as estimated for wild-type and DNA repair mutants with elevated SV rates. C. Size distributions of tandem duplications (top, pink) and deletions (bottom, green) across wild-type and mutants with elevated SV rates. D. Clustering of mutations in DNA repair deficient mutants. Grey dots reflect the average proportions of clustered mutations. Error bars denote 95% confidence intervals. Mutants with a significantly different propensity for mutation clustering from wild-type (dotted black line) are shown and highlighted in red. ‘Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Journal: PLoS ONE

Article Title: Protection of the C . elegans germ cell genome depends on diverse DNA repair pathways during normal proliferation

doi: 10.1371/journal.pone.0250291

Figure Lengend Snippet: A. Mutational signatures of DSBR mutants that exhibited statistically significant different mutation rates to wild-type displayed in numbers of mutations per generation. Bold coloured bars denote individual mutation classes where the number of mutations is different from wild-type, an underscore below each mutation profile indicates mutation types with total mutation numbers different from wild-type, and three stars indicate genotypes which have rates of substitutions, indels or SVs significantly different compared to wild-type (FDR < 5%). B. Estimated composition of structural variants per generation as estimated for wild-type and DNA repair mutants with elevated SV rates. C. Size distributions of tandem duplications (top, pink) and deletions (bottom, green) across wild-type and mutants with elevated SV rates. D. Clustering of mutations in DNA repair deficient mutants. Grey dots reflect the average proportions of clustered mutations. Error bars denote 95% confidence intervals. Mutants with a significantly different propensity for mutation clustering from wild-type (dotted black line) are shown and highlighted in red. ‘Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Article Snippet: In summary, DNA sequencing was performed using Illumina HiSeq 2000 and 10X Genomics short reads sequencing platforms at 100 bp paired-end, with a mean coverage of 50x.

Techniques: Mutagenesis, Sequencing

A. Mutational signatures of TLS and ICLR mutants that exhibited statistically significant differences to wild-type mutation rates displayed in numbers of mutations per generation. Same layout as . B . Proportion of indels (brown) and SVs (black) in G-rich regions in wild-type and across genotypes with elevated rates of SVs. Dotted line represents the proportion of variants falling into these regions as expected by chance. C . Tandem duplications (TDs) in helq-1 mutants. An analysis of rev-3 was previously shown in . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Journal: PLoS ONE

Article Title: Protection of the C . elegans germ cell genome depends on diverse DNA repair pathways during normal proliferation

doi: 10.1371/journal.pone.0250291

Figure Lengend Snippet: A. Mutational signatures of TLS and ICLR mutants that exhibited statistically significant differences to wild-type mutation rates displayed in numbers of mutations per generation. Same layout as . B . Proportion of indels (brown) and SVs (black) in G-rich regions in wild-type and across genotypes with elevated rates of SVs. Dotted line represents the proportion of variants falling into these regions as expected by chance. C . Tandem duplications (TDs) in helq-1 mutants. An analysis of rev-3 was previously shown in . Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Article Snippet: In summary, DNA sequencing was performed using Illumina HiSeq 2000 and 10X Genomics short reads sequencing platforms at 100 bp paired-end, with a mean coverage of 50x.

Techniques: Mutagenesis, Sequencing

A. Mutational signatures of mutants that exhibited statistically significant differences to wild-type mutation rates. The chromosomes on which respective genes are located are indicated in superscript following each mutant name. Layout as . B. Proportion of SVs with breakpoints into subtelomeric regions across wild-type and mutants that exhibit elevated SV rates. Dotted lines represent the fraction of variants expected to occur in subtelomeric regions by chance. C . Examples of subtelomeric structural variants in atm-1 mutants. D. Quantification of mutation burden in indicated DNA repair mutants for initial generations and F20 and F40 generations as shown. Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Journal: PLoS ONE

Article Title: Protection of the C . elegans germ cell genome depends on diverse DNA repair pathways during normal proliferation

doi: 10.1371/journal.pone.0250291

Figure Lengend Snippet: A. Mutational signatures of mutants that exhibited statistically significant differences to wild-type mutation rates. The chromosomes on which respective genes are located are indicated in superscript following each mutant name. Layout as . B. Proportion of SVs with breakpoints into subtelomeric regions across wild-type and mutants that exhibit elevated SV rates. Dotted lines represent the fraction of variants expected to occur in subtelomeric regions by chance. C . Examples of subtelomeric structural variants in atm-1 mutants. D. Quantification of mutation burden in indicated DNA repair mutants for initial generations and F20 and F40 generations as shown. Information related to the 528 whole genome sequencing WGS primary-source datasets (56 deposited in this study, 472 deposited in (Suppl Data 1 and Supple Note 1 of can be found in ).

Article Snippet: In summary, DNA sequencing was performed using Illumina HiSeq 2000 and 10X Genomics short reads sequencing platforms at 100 bp paired-end, with a mean coverage of 50x.

Techniques: Mutagenesis, Sequencing

RNA vaccines against influenza virus.*

Journal: Vaccines

Article Title: New Kids on the Block: RNA-Based Influenza Virus Vaccines

doi: 10.3390/vaccines6020020

Figure Lengend Snippet: RNA vaccines against influenza virus.*

Article Snippet: CureVac AG developed a sequence-engineered mRNA-LNP platform that enables a high level of in vivo protein translation without the use of modified nucleosides [ ].

Techniques: Infection