skiingfiend• in reply toMaxone734 months ago

I have had 2 ctDNA tests run under a research protocol. Here are the results to give you a feel for what can be reported. ctDNA tests are used to identify point-in-time somatic mutations which may be related to specific treatment options. ctDNA enables personalized medicine which more specifically targets your cancer and its mutations than systemic therapy.

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To date, we have sequenced two of your samples: 8/NOV/2022 (just prior to you starting ADT injections) and 13/FEB/2024 (when you developed liver metastases).

1. Germline mutations

We saw the germline CHEK2 mutation that you inherited. This was expectedly observed in both samples (your germline DNA doesn't change over time).

2. Tumour fraction

Think of this as the proportion of the free-floating DNA in your blood that is tumour-derived. In the first sample, it was ~10%. In the second sample, it was ~40%. Note: these are merely estimates, there is a degree of uncertainty around these results. I think the main take home message is the tumour fraction did go up significantly between your first and second sample. Of course, this fits with what we saw on your scans. Another thing to be aware of is that an increase from 10% to 40% does not mean that the amount of cancer has increased four-fold. It just means that the tumour is dividing at a faster rate at the time of the second sample compared to when we took the first sample. Again, this seems consistent with the diagnosis of small cell prostate cancer.

3. Somatic mutations

- In the first sample, we saw mutations in CTNNB1 (Missense p.S33A), KMT2C (Stopgain p.Q957X), KDM6A (Frameshift p.F62Wfs*16), and KDM6A (Stopgain p.S1348X).

- In the second sample: despite an increase in the overall tumour fraciton, we were only able to 'rediscover' the KMT2C (Stopgain p.Q957X) mutation. It suggests that the cancer cells carrying the CTNNB1 and 2 x KDM6A mutations were wiped out from your original treatment (or are still present but a very, very low level), but the cancer cell population harbouring the KMT2C mutation has persisted and risen to be the dominant clone. No other mutations were seen in this second sample.

- None of these mutations described in this Somatic mutation section are clinically actionable. That is, none of them are directly tied to any specific targeted therapy.

4. Other alterations

- We saw evidence that your tumour had lost all copies of PTEN, which is a tumour suppressor gene. We do see this in small cell prostate cancer, and can be accompanied by genomic alterations in TP53 and RB1. We did not see any biologically relevant alterations in TP53 and RB1 from your tumour.

- Tumours with PTEN deletion cause activation of the PI3K pathway, which is a major growth pathway. Hyperactivation of the PI3K pathway is potentially targetable with inhibitors against this pathway. Some of them in testing include capivasertib (AKT inhibitor) and ipatasertib (AKT inhibitor clinical development was halted last year though unfortunately). These drugs have been tested in prostate adenocarcinoma (attached most relevant paper) - there really isn't any data to support its use in small cell prostate cancer.

Note: these results are research findings only, and technically can't be used to directly inform your care unless there is confirmatory clinical grade testing.

All in all, I don't think the genomic testing you performed adds any additional information to inform your care. It was critical to perform, but I would stay on the current treatment, and focus on small cell therapies.

garyjp9• in reply toMaxone734 months ago

Thank you

garyjp9• in reply toMaxone734 months ago

thank you