| 1. |
- Ameur, Adam, et al.
(författare)
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SweGen : a whole-genome data resource of genetic variability in a cross-section of the Swedish population
- 2017
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Ingår i: European Journal of Human Genetics. - : NATURE PUBLISHING GROUP. - 1018-4813 .- 1476-5438. ; 25:11, s. 1253-1260
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Tidskriftsartikel (refereegranskat)abstract
- Here we describe the SweGen data set, a comprehensive map of genetic variation in the Swedish population. These data represent a basic resource for clinical genetics laboratories as well as for sequencing-based association studies by providing information on genetic variant frequencies in a cohort that is well matched to national patient cohorts. To select samples for this study, we first examined the genetic structure of the Swedish population using high-density SNP-array data from a nation-wide cohort of over 10 000 Swedish-born individuals included in the Swedish Twin Registry. A total of 1000 individuals, reflecting a cross-section of the population and capturing the main genetic structure, were selected for whole-genome sequencing. Analysis pipelines were developed for automated alignment, variant calling and quality control of the sequencing data. This resulted in a genome-wide collection of aggregated variant frequencies in the Swedish population that we have made available to the scientific community through the website https://swefreq.nbis.se. A total of 29.2 million single-nucleotide variants and 3.8 million indels were detected in the 1000 samples, with 9.9 million of these variants not present in current databases. Each sample contributed with an average of 7199 individual-specific variants. In addition, an average of 8645 larger structural variants (SVs) were detected per individual, and we demonstrate that the population frequencies of these SVs can be used for efficient filtering analyses. Finally, our results show that the genetic diversity within Sweden is substantial compared with the diversity among continental European populations, underscoring the relevance of establishing a local reference data set.
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| 2. |
- Hård, Joanna, et al.
(författare)
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Long-read whole-genome analysis of human single cells
- 2023
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Ingår i: Nature Communications. - : Springer Nature. - 2041-1723. ; 14:1
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Tidskriftsartikel (refereegranskat)abstract
- Long-read sequencing has dramatically increased our understanding of human genome variation. Here, we demonstrate that long-read technology can give new insights into the genomic architecture of individual cells. Clonally expanded CD8+ T-cells from a human donor were subjected to droplet-based multiple displacement amplification (dMDA) to generate long molecules with reduced bias. PacBio sequencing generated up to 40% genome coverage per single-cell, enabling detection of single nucleotide variants (SNVs), structural variants (SVs), and tandem repeats, also in regions inaccessible by short reads. 28 somatic SNVs were detected, including one case of mitochondrial heteroplasmy. 5473 high-confidence SVs/cell were discovered, a sixteen-fold increase compared to Illumina-based results from clonally related cells. Single-cell de novo assembly generated a genome size of up to 598 Mb and 1762 (12.8%) complete gene models. In summary, our work shows the promise of long-read sequencing toward characterization of the full spectrum of genetic variation in single cells.
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| 3. |
- Höjer, Pontus
(författare)
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Exploring human variations by droplet barcoding
- 2024
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Doktorsavhandling (övrigt vetenskapligt/konstnärligt)abstract
- Biological variations are being explored at ever-increasing rates through the rapid advancement of analytical techniques. Techniques like massively parallel sequencing empower scientists to accurately differentiate individuals’ genetic compositions, cellular functionalities, and healthy tissue from diseased. The knowledge gained from these techniques brings us ever closer to grasping the complexities of life, contributing to human development. Still, to fully elucidate biological variations in different samples requires novel sensitive and high- throughput techniques, capable of placing everything in its correct context. One such technique gaining promise is droplet barcoding. Droplet barcoding leverages emulsion droplets to segregate samples into their functional components, coupled with barcodes that can group tagged molecules following sequencing. This technique constitutes a versatile tool for studying biological variations in both the phenotype and genotype. This thesis leverages droplet barcoding to explore variations relating to human biology. Droplet barcoding was used to study phenotype variations, looking at protein compositions in single extracellular vesicles (Paper I) and single cells (Paper II). Paper I studies extracellular vesicles which are naturally released from cells. They carry heterogeneous protein signatures that can inform about their cellular origin. Tens of thousands of extracellular vesicles were profiled, including approximately 25,000 from lung cancer patients. From these protein profiles, extracellular vesicles could be grouped into putative subtypes. Paper II presents a novel method for studying single cells which was used to characterize blood-derived immune cells. The method enabled the identification of most major immune cell lineages. Haplotype-resolved genetic variations were analyzed using a linked read sequencing method based on droplet barcoding. Linked-read sequencing conserves long-range information from short-read sequencing by co- barcoding subsections of long DNA fragments. Paper III presents an open-source pipeline (BLR) for whole genome haplotyping using linked reads. BLR generates accurate and continuous haplotypes, outperforming PacBio HiFi-based diploid assembly. We further show that integration with low-coverage long-read data can improve phasing accuracy in tandem repeats. With 10X Genomics linked reads, BLR generated more continuous haplotypes compared to other workflows. Paper IV applies linked read sequencing to reveal the haplotype complexities of cancer genomes. In two patients with colorectal cancer, we identified several large-scale aberrations impacting cancer-related genes. Additionally, several short somatic variants were found to impact nearly all oncogenic networks identified by TCGA. Demonstrating the importance of haplotype-resolved analysis for cancer genomics, one patient exhibited two nonsense mutations on separate haplotypes in the well-known colorectal cancer gene APC.
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| 4. |
- Just, David, et al.
(författare)
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Exploring autoantibody signatures in brain tissue from patients with severe mental illness
- 2020
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Ingår i: Translational Psychiatry. - : Springer Nature. - 2158-3188. ; 10:1
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Tidskriftsartikel (refereegranskat)abstract
- In recent years, studies have shown higher prevalence of autoantibodies in patients with schizophrenia compared to healthy individuals. This study applies an untargeted and a targeted affinity proteomics approach to explore and characterize the autoantibody repertoire in brain tissues from 73 subjects diagnosed with schizophrenia and 52 control subjects with no psychiatric or neurological disorders. Selected brain tissue lysates were first explored for IgG reactivity on planar microarrays composed of 11,520 protein fragments representing 10,820 unique proteins. Based on these results of ours and other previous studies of autoantibodies related to psychosis, we selected 226 fragments with an average length of 80 amino acids, representing 127 unique proteins. Tissue-based analysis of IgG reactivities using antigen suspension bead arrays was performed in a multiplex and parallel fashion for all 125 subjects. Among the detected autoantigens, higher IgG reactivity in subjects with schizophrenia, as compared to psychiatrically healthy subjects, was found against the glutamate ionotropic receptor NMDA type subunit 2D (anti-GluN2D). In a separate cohort with serum samples from 395 young adults with a wider spectrum of psychiatric disorders, higher levels of serum autoantibodies targeting GluN2D were found when compared to 102 control individuals. By further validating GluN2D and additional potential autoantigens, we will seek insights into how these are associated with severe mental illnesses.
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| 5. |
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| 6. |
- Kvastad, Linda
(författare)
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The Spatial Context – through the lens of method development
- 2021
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Doktorsavhandling (övrigt vetenskapligt/konstnärligt)abstract
- In the present moment of time, we find ourselves in a period where the advancement of genomic tools is progressing at a fast pace. Of particular interest for this thesis is the study of gene activity. What patterns of genes are expressed? Where are they expressed? How can we use this knowledge to improve our quality of life? The research presented in this thesis focuses on developing and applying new tools for interrogating cells and tissues. In Paper I, we describe a protocol for transcript profiling of single cells, capable of measuring the relative expression levels for genes of interest. We successfully applied our method to cancer cells from metastatic breast cancer patients. Profiling 2 to 4 single cells per patient and measuring gene-specific expression from targets previously associated with metastatic breast cancer supports the use of our protocol as a diagnostic tool. In Paper II, we present an assay for spatial RNA quality evaluation, used to estimate the success for tissue specimens before proceeding with more expensive spatial sequencing methods. We showed that the method is capable of measuring high RNA quality in tissue areas of both high and low cell density and that the spatial RNA integrity patterns are reflected in spatial transcriptomics data. In Paper III, we present a protocol for performing spatial mRNA genome-wide expression profiling of FFPE tissue specimens. Thus, we bridge a gap between traditional tissue preservation methods and novel gene technologytools. We found a high Pearson correlation of 0.95 between formalin-fixation paraffin embedding (FFPE) and Fresh Frozen (FF) mouse brain datasets. Although the FPPE samples yielded fewer transcripts and genes compared to FF, there was a high agreement in gene expression between paired anatomical areas for FFPE and FF samples. In Paper IV, we present an approach to investigate in situ transcript derivedinferred copy number variation (iCNV) profiles based on spatial transcriptomics data. In a normal lymph node that displays both distinct gene expression patterns and histological landmarks, we observed a neutral iCNV profile. In contrast, we found huge variabilities investigating several malign tissue types ranging from homogenous (pediatric medulloblastoma) to highly variable genomes (ductal breast cancer and glioblastoma). Strikingly, we also observed similar iCNV profiles in both tumor and benign tissue areas from prostate and skin cancer. In Paper V, we explore the transcriptional and genomic landscape in pediatric tumors from 14 patients. Microglia cells have been implicated to play an important role in the tumor microenvironment, and we found spatial co-localization of microglia and epithelial-to-mesenchymal transition (EMT) signatures in our patient cohort. Furthermore, we found homogenous and recurrent iCNV profiles in the high-grade tumors of relapse patients and identified expression of gene SPP1 in the tumor stroma as a potential prognostic mRNA marker in pediatric brain tumor relapse patients.
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