Natural killer cells (NK) are effector cells of innate immune system. Their key role is to recognise and destroy cancerous, virus infected and fungus infected cells in humans. They are also an early source of proinflammatory cytokines, especially interferon ? (IFN-?) and chemokines that activate and attract other immune cells. There are two main subpopulations of NK cells in peripheral blood, distinctly cytotoxic subpopulation of CD56Pdim PNK cells and mostly regulatory CD56PbrightP NK cells that are an important source of early IFN-?. NK cell activity (NKA) can be determined by in vitro measuring of released IFN-? as well as with a direct cytotoxicity assay using model target cells. NKA in healthy individuals is relatively stable through longer periods of time and the ratio between NK subpopulations remains mostly unchanged. In clinical studies it is reported that in patients with prostate cancer, NKA decreases with advancing cancer stage. These studies are accompanied with reports of diminishing subpopulation of CD16P-PCD56Pbright Pin peripheral blood, which promotes a stronger immune response against cancer cells. In our work we measured cytotoxic NKA in samples of cells acquired from PBMC of six patients with prostate cancer in different time points during a clinical trial of an anticancer immune therapy. The percentages of cytotoxicity were measured in in vitro conditions on the basis of results from a direct cytotoxicity assay based on the amount of released intracellular enzyme lactate dehydrogenase (LDH) from killed target cells K562. We used a letter V shaped 96 well microtiter plates for performing the assay on the basis of preliminary testing. In two patients we also performed a cytotoxic assay using flow cytometry, where we dyed the target cells K562 with CFSE and 7-AAD dyes. Flow cytometry is a good alternative to LDH assay because we can determine the cytotoxicity on a single cell level with this technique. Our results mainly show large variations in NKA through the course of our clinical trial compared to our control values of samples taken before the first application of the trial substances, which is most likely a consequence of before mentioned therapy. Patients tested for NKA were representing three groups based on their responsiveness to antitumor therapy based on defined clinical parameters. We could not prove a correlation between NKA and clinical outcomes with our limited study subjects, but we observed trends which could in a large enough sample prove a correlation between the two. We would also need to design our clinical study for this purpose and take samples during a longer period of time, especially after the end of experimental treatment.