Disrupting cellular memory to overcome drug resistance
Posted on: 18 September 2022 , updated on: 18 March 2024
Preprint posted on 5 August 2022
Article now published in Nature Communications at http://dx.doi.org/10.1038/s41467-023-41811-8
Categories: bioinformatics, cell biology, genetics, genomics, molecular biology
Updated 18 March 2024 with a postLight by Nate Mullin
A version of this study by Harmange and colleagues is now published in Nature Communications, a bit over a year after the preprint was initially posted on bioRxiv. The initial work was quite robust, and both introduced and validated a new technique, scMemorySeq, and demonstrated its utility in a clinically relevant model of drug resistance in cancer cells.
The main changes to the paper during the peer review process appear to revolve around the organization and logical presentation of experiments. In the preprint, Figure 1 both introduced scMemorySeq and showed data from a drug treatment experiment demonstrating that cell state switching prior to treatment could alter the survival dynamics of a population. In the Nature Communications paper, this experiment has been moved to the last primary figure (Figure 6) and is presented with a couple of additional conditions. Figure 6 now shows how cell states can be modulated in either direction by drugging pathways identified in previous figures.
The order of Figures 2 and 3 has also been flipped. I believe these changes help to create a new logic to the paper in which cell states (primed vs drug-susceptible) are first observed using scMemorySeq, then validated through other tumor models, followed by molecular dissection of their differences and leveraging these differences to show state modulation in the final figure.
The peer review file from Nature Communications is also available for this paper and contains an informative discussion between authors and reviewers on both the points I have discussed here and on analytical methods that were used (and shown in supplemental figures) to strengthen the conclusions of the paper.
Background
Is there a way to understand, or even predict, the seemingly random behavior of certain cells? If so, how could such an understanding be leveraged to combat insidious cellular behaviors such as chemotherapy resistance?
In normal development and in disease states like cancer, the character of individual cells is malleable. Two descriptions of what a cell may be able to do at any particular time are cell state and cell type. While the exact distinction between these categories remains open to debate, cell type is generally regarded as a permanent description based on developmental lineage and function. Cell state exists on the opposite end of the permanence spectrum and can be thought of as a transient set of characteristics taken up by a cell, perhaps in response to an external stimulus or perhaps due only to random chance.
The preprint by Harmange et al. focuses on a type of cellular identity that sits in between these two extremes: cell memory. Shaffer and colleagues previously described cell memory as a heritable (across cell division), yet impermanent feature of a cell. For example, gene expression memory would describe a state of gene expression present in a cell for a certain amount of time that might even be passed into daughter cells yet is not part of the core program that defines the cell’s identity (i.e., once the transient time period ends, the cell would not lose its identity nor cease to be that type).
In the context of cancer, gene expression memory states have important clinical implications. Cell memory may confer drug resistance to certain lineages of cells, leading to growth of drug-resistant tumors after chemotherapy. Because of the transient nature of gene expression memory, these states are not genetically encoded, and may be gained or lost in particular lineages across time. Harmange et al. used the well-described melanoma model of drug resistance to BRAF and MEK inhibitors to define memory states of cancer cells primed to resist or succumb to drug treatment. They then went on to experimentally identify the pathway that allows state switching in these cells prior to drug treatment.
Key findings
Single-cell memory sequencing (scMemorySeq) combines cellular lineage tracing with gene expression profiling through transient cell state transitions.
In order to understand the transcriptional landscape of cells in different states (i.e. primed for drug resistance or susceptible to treatment) and to track lineages of cells that transition between states, the authors developed scMemorySeq (Figure 1). This technique combines lineage tracing via lentiviral barcoding with phenotyping and single-cell gene expression analysis. ScMemorySeq allows the past behavior of a cell to be linked to its current cell state.
Lineages that switch between susceptible and resistance-primed states are transcriptomically distinct from those that do not.
Related cells (i.e. with a common progenitor) can change state to either gain or lose the transcriptional profile associated with drug susceptibility. By comparing lineages of cells that make this switch to lineages that do not, key genes involved in state conversion can be identified (Figure 2). These can be aggregated into a gene expression module (“crossing lineage score”) that individual cells can be scored on. The authors identified epithelial mesenchymal transition (EMT)-related genes as enriched in state-switching lineages.
Modulation of drug-response behavior through targeting of transition-mediating pathways.
The authors targeted the pathways involved in state switching identified by scMemorySeq using agonists and antagonists of the TGFB and PI3K pathways. Inhibition of PI3K in a mixed population of primed and susceptible cells led to a decrease in the proportion of primed cells, whereas activation of TGFB signaling increased the proportion of primed cells (Figure 3). Transcriptionally, newly primed or susceptible cells resembled those without treatment (Figure 3F).
PI3K modulation increases the proportion of drug-susceptible cells through state-switching.
State-switching behavior was modeled using a simulation taking into account three parameters: the rate of state switching, the rate of cell death, and the rate of cell division. The authors found that an increased rate of state switching best explained their experimental data. This finding supports the hypothesis that drug treatment alters population dynamics through increased switching, not by killing off certain populations. The authors could finally show that pre-treatment with state-switching drugs does in fact increase the effectiveness of BRAFi/MEKi treatment against drug-naïve melanoma cells in vitro.
What I like about this work
In recent years, single-cell genomic and transcriptomic techniques have put the spotlight on cellular heterogeneity in the context of disease and normal physiology. However, such are mostly restricted to a single point in time. This means that while we can observe sub-populations of cells within a tissue, we cannot know how they have in the past or would in the future react to particular insults or unique environments. Such knowledge is essential for understanding how disease develops (e.g. why are some, but not all cells of a certain type affected by a genetic variant) and how transient subpopulations could best be targeted in the treatment of disease
In this preprint, the authors have demonstrated how scMemorySeq can be used to overcome this temporal hurdle. They showed that even within validated clusters, pre-fated trajectories are coded into individual cells. As a reader and researcher interested in genetic disease, the concept that these fate trajectories are knowable and detectable with current technology shifts how I think about cellular heterogeneity.
Questions for authors
- Is state-switching itself a lineage-specific phenomenon? Do certain lineages switch states more frequently than others?
- Similarly, what do you think changes a lineage’s ability to switch states? Could this be genetically encoded, or are all cells genetically identical?
- Are transient gene expression memory states important outside of cancer? Do you think that these underly cell fate decisions in normal development?
doi: https://doi.org/10.1242/prelights.32390
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