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Single-cell analysis: toward the clinic

Human life starts with a single cell, the zygote, which undergoes multiple mitotic cell divisions to form a complete body. During each cell division, the genome has to be replicated to form the approximately 1014 cells that make up the adult human body. For a long time, it was thought that all cells from the same individual harbored identical genomes. The only known exceptions being lymphocytes, in which antigen- and pathogen-driven recombination and hypermutation generate genetic diversity, and germline cells, which undergo meiotic recombination.

During normal mitotic cell division, however, the genome is not replicated with absolute precision; this results in the incorporation of somatic mutations [1]. Estimates that are based on known mutation rates suggest that every cell division creates some form of genetic variation, which may or may not have an effect on cellular function [2, 3]. During the progression from the zygotic stage to adulthood, these somatic mutations accumulate (Figure 1). Recent genome-wide assays have suggested that an individual does not have one genome, but is instead made up of a population of different cells. This situation is referred to as mosaicism, that is, the co-occurrence of several cell lineages with different genotypes in one individual who has developed from a single fertilized egg. The true extent of such mosaicism is unknown, but its presence appears to be the rule rather than the exception [4]. Estimates of the mutation burden in somatic cells are high and, as a consequence, it has been speculated that each cell in a human body may have a unique genomic signature; in other words, that each cell has its own 'personal genome' [4, 5].

Figure 1
figure 1

A schematic representation of the effects of somatic mutations at different phases of development and tissue renewal. Life starts from a single cell, a fertilized egg (blue circle). A complete organism, that is a human, is formed from this cell by many cell divisions. Novel somatic mutations can occur with each cell division. The diagram shows how such mutations are passed on to daughter cells as the organism develops: a mutation may undergo clonal expansion during tissue renewal. If the somatic mutation occurs late (brown clones), the mutation will be found in only a small compartment of the body, that is, it is likely to be confined to one organ. If the mutation occurs very early in development - for example, during embryogenesis (dark blue clones) - it is likely to occur in different organs. Successive mutations, which can then establish organismal cell lineage trees, can occur in cells derived from those that underwent an early mutation (clones in lighter blue color within the dark blue clone). The serial acquisition of novel mutations is shown as an example for the first series of blue clones (red bases). Some mutations may be disadvantageous and go extinct (black clones). (Image adapted in part from [6].)

Many of these mutations will be neutral, in other words, they do not result in a selective advantage or disadvantage for the cell (Figure 1). On the other hand, some mutations may affect genes, and subsequently transcription and protein synthesis. The exact range of the possible biological functions of such somatic mutations is hard to grasp. Some somatic mutations are instrumental in causing diseases, especially cancers [6], or for the physiologic process of aging [7]. The apparently large extent of somatic mosaicism suggests, however, that some mutations may have normal physiological functions [4]. For example, the brain appears to harbor widespread somatic mutations in the form of aneuploidy or retrotransposon insertions, and it has been speculated that this extensive somatic genome mosaicism might contribute to normal brain function [8, 9].

The extent of genetic mosaicism has tremendous implications for both basic research and clinical applications. Despite Virchow's discovery more than 150 years ago that the single cell represents the basic unit of disease [10], research and diagnostics are usually performed on thousands of cells without considering the different cell lineages in a body. Such a diagnostic provides only average information about the cells examined.

The usual source of cells for clinical diagnostics is the peripheral blood because of its easy accessibility. In cases of suspected mosaicism, the usual diagnostics include additional analyses of non-hematogenous cells, which are obtained by skin biopsies and/or buccal swabs, or the analyses of paired samples of visibly affected and normal tissue. The latter strategy resulted, for example, in the identification of somatic AKT1 mutations as the cause of Proteus syndrome [11] and of somatic GNAQ mutations in individuals with Sturge-Weber syndrome [12]. In the case of unaffected parents who have an affected child, human geneticists have to consider the option that one parent has a germline mosaic, which would affect the recurrence risk for the affected child's sibling. Nevertheless, germline mosaics are rarely analyzed further as germ cells are difficult to obtain from females.

To understand a complex phenotype, large-scale, whole-body single-cell-type analyses, including the characterization of genomics, transcriptomics, proteomics, and epigenomics are needed. Such analyses would greatly contribute to an improvement of our fundamental understanding of both biology and medicine. Furthermore, they would most probably reveal multiple novel insights into disease occurrence and aging.

How could such analyses of single-cells from various tissue types be performed? One suggestion is a more detailed analysis of all surgically excised tissues, including tonsils, appendices, defective heart valves, skeletal muscle, and normal tissue in the proximity of tumors [4]. If this material were obtained in a viable form, somatic cells could be reprogrammed in order to generate induced pluripotent stem cells (iPSCs). For example, widespread somatic mosaicism that results from acquired post-zygotic structural alterations in human skin has recently been detected by whole-genome and transcriptome analysis of iPSCs derived from primary skin fibroblasts [13]. The derivation of iPSCs is attractive as it offers the opportunity to examine single cells at many levels - genomics, proteomics, transcriptomics, metabolomics and systems biology - at high resolution and sensitivity. In addition to iPSCs, multiple novel single-cell techniques have emerged in recent years, making the genome, transcriptome and proteome of single cells accessible to detailed analyses. Many of these novel methods are discussed in various contributions in this series of articles for Genome Medicine.

With the current progress in developing sophisticated single-cell approaches, what biological and medical questions can be addressed? First, single-cell analyses will improve our understanding of intercellular variability and its biological consequences in connection with disease susceptibility and aging. Second, single-cell analyses might contribute to a better definition of cell types. At present, the classification of cell types is based on characteristics, such as morphology, genotype, phenotype, or developmental origin. There is no common agreement on what really defines a cell type [5]. Hence, large-scale single-cell transcriptome or epigenome analyses might result in an improved definition of cell types and could also help to identify rare cell types [5]. Third, the strength of single-cell technologies lies in their ability to analyze rare cell events. For example, for patients with cancer, single-cell technologies are playing an increasing role in the detection of minimal residual disease or in the analysis of circulating tumor cells in the peripheral blood. Fourth, single-cell technologies are already instrumental in pre-implantation diagnosis, where just one or two cells from the blastocyst are commonly subjected to analysis. Finally, single-cell technologies will contribute to unraveling the true extent of single-cell somatic mutations. This will make it possible to use the accumulation of mutations in single cells during development to infer the lineage ancestry of each cell (Figure 1), which will answer important questions in human biology and medicine [5].

At present, the clinical use of single-cell analysis is - with the exception of pre-implantation diagnosis - still in its infancy. For the reasons mentioned above, however, single-cell diagnostics will be instrumental for the realization of personalized medicine and for the development of completely novel therapeutic concepts. Hence, the bold prediction has been made that we are facing an era of integrated single-cell genomic, epigenomic, transcriptomic, and proteomic analysis that will revolutionize whole-organism science [5].

Abbreviations

iPSC:

induced pluripotent stem cell.

References

  1. Poduri A, Evrony GD, Cai X, Walsh CA: Somatic mutation, genomic variation, and neurological disease. Science. 2013, 341: 1237758-10.1126/science.1237758.

    Article  PubMed  PubMed Central  Google Scholar 

  2. Frumkin D, Wasserstrom A, Kaplan S, Feige U, Shapiro E: Genomic variability within an organism exposes its cell lineage tree. PLoS Comput Biol. 2005, 1: e50-10.1371/journal.pcbi.0010050.

    Article  PubMed  PubMed Central  Google Scholar 

  3. Lynch M: Evolution of the mutation rate. Trends Genet. 2010, 26: 345-352. 10.1016/j.tig.2010.05.003.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

  4. Lupski JR: Genetics. Genome mosaicism - one human, multiple genomes. Science. 2013, 341: 358-359. 10.1126/science.1239503.

    Article  CAS  PubMed  Google Scholar 

  5. Shapiro E, Biezuner T, Linnarsson S: Single-cell sequencing-based technologies will revolutionize whole-organism science. Nat Rev Genet. 2013, doi: 10.1038/nrg3542

    Google Scholar 

  6. Tomasetti C, Vogelstein B, Parmigiani G: Half or more of the somatic mutations in cancers of self-renewing tissues originate prior to tumor initiation. Proc Natl Acad Sci USA. 2013, 110: 1999-2004. 10.1073/pnas.1221068110.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

  7. Lopez-Otin C, Blasco MA, Partridge L, Serrano M, Kroemer G: The hallmarks of aging. Cell. 2013, 153: 1194-1217. 10.1016/j.cell.2013.05.039.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

  8. Baillie JK, Barnett MW, Upton KR, Gerhardt DJ, Richmond TA, De Sapio F, Brennan PM, Rizzu P, Smith S, Fell M, Talbot RT, Gustincich S, Freeman TC, Mattick JS, Hume DA, Heutink P, Carninci P, Jeddeloh JA, Faulkner GJ: Somatic retrotransposition alters the genetic landscape of the human brain. Nature. 2011, 479: 534-537. 10.1038/nature10531.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

  9. Evrony GD, Cai X, Lee E, Hills LB, Elhosary PC, Lehmann HS, Parker JJ, Atabay KD, Gilmore EC, Poduri A, Park PJ, Walsh CA: Single-neuron sequencing analysis of L1 retrotransposition and somatic mutation in the human brain. Cell. 2012, 151: 483-496. 10.1016/j.cell.2012.09.035.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

  10. Virchow RLK: Die Cellularpathologie in ihrer Begründung auf physiologische und pathologische Gewebelehre. Berlin: A Hirschwald. 1858

    Google Scholar 

  11. Lindhurst MJ, Sapp JC, Teer JK, Johnston JJ, Finn EM, Peters K, Turner J, Cannons JL, Bick D, Blakemore L, Blumhorst C, Brockmann K, Calder P, Cherman N, Deardorff MA, Everman DB, Golas G, Greenstein RM, Kato BM, Keppler-Noreuil KM, Kuznetsov SA, Miyamoto RT, Newman K, Ng D, O'Brien K, Rothenberg S, Schwartzentruber DJ, Singhal V, Tirabosco R, Upton J, et al: A mosaic activating mutation in AKT1 associated with the Proteus syndrome. N Engl J Med. 2011, 365: 611-619. 10.1056/NEJMoa1104017.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

  12. Shirley MD, Tang H, Gallione CJ, Baugher JD, Frelin LP, Cohen B, North PE, Marchuk DA, Comi AM, Pevsner J: Sturge-Weber syndrome and port-wine stains caused by somatic mutation in GNAQ. N Engl J Med. 2013, 368: 1971-1979. 10.1056/NEJMoa1213507.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

  13. Abyzov A, Mariani J, Palejev D, Zhang Y, Haney MS, Tomasini L, Ferrandino AF, Rosenberg Belmaker LA, Szekely A, Wilson M, Kocabas A, Calixto NE, Grigorenko EL, Huttner A, Chawarska K, Weissman S, Urban AE, Gerstein M, Vaccarino FM: Somatic copy number mosaicism in human skin revealed by induced pluripotent stem cells. Nature. 2012, 492: 438-442. 10.1038/nature11629.

    Article  CAS  PubMed  PubMed Central  Google Scholar 

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Acknowledgements

I thank Mag. Maria Langer-Winter for editing the manuscript. Funding in the author's laboratory was provided by the Austrian Science Fund (FWF) (grant numbers: P20338, P23284 and W 1226-B18, DKplus Metabolic and Cardiovascular Disease), and the Oesterreichische Nationalbank (grant number: 15093).

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Correspondence to Michael R Speicher.

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Speicher, M.R. Single-cell analysis: toward the clinic. Genome Med 5, 74 (2013). https://doi.org/10.1186/gm478

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