Decoding the mechanism behind MCL-1 inhibitors: A pathway to understanding MCL-1 protein stability

The diversity of BH3 proteins can be broadly characterized as pro-survival (BCL-2, MCL-1, BCLxL, Bfl-1/A1, Bcl-w, Bcl-b) or pro-apoptotic (Bax, Bak; and Bim, Puma, BID, BAD, BIK, HRK, BMF, Noxa). Pro-survival proteins function by sequestering the proapoptotic proteins, thus preventing the initiation of an apoptotic cascade. However, overexpression of prosurvival proteins can help in tumorigenesis and drug resistance, making them an attractive target for inducing apoptosis in cancer cells [1]. The successful development of BCL-2 inhibitor (venetoclax), currently approved for chronic lymphocytic leukemia (CLL) and acute myeloid leukemia (AML), encouraged the development of inhibitors that target other antiapoptotic proteins, particularly Myeloid Leukemia 1 (MCL-1). MCL-1 is among the top genes amplified in several cancers and is implicated in cancer progression, drug resistance and poor prognosis. It protects cancer cells from

The diversity of BH3 proteins can be broadly characterized as pro-survival (BCL-2, MCL-1, BCL-xL, Bfl-1/A1, Bcl-w, Bcl-b) or pro-apoptotic (Bax, Bak; and Bim, Puma, BID, BAD, BIK, HRK, BMF, Noxa). Pro-survival proteins function by sequestering the proapoptotic proteins, thus preventing the initiation of an apoptotic cascade. However, overexpression of prosurvival proteins can help in tumorigenesis and drug resistance, making them an attractive target for inducing apoptosis in cancer cells [1]. The successful development of BCL-2 inhibitor (venetoclax), currently approved for chronic lymphocytic leukemia (CLL) and acute myeloid leukemia (AML), encouraged the development of inhibitors that target other antiapoptotic proteins, particularly Myeloid Leukemia 1 (MCL-1).
MCL-1 is among the top genes amplified in several cancers and is implicated in cancer progression, drug resistance and poor prognosis. It protects cancer cells from apoptosis and decreases their sensitivity to targeted agents or chemotherapeutics [2][3][4][5][6]. MCL-1 preferentially binds to Bak and Noxa, thus inhibiting the release of cytochrome C and activation of the apoptotic cascade. Besides, MCL-1 performs other functions including DNA repair, cell cycle regulation, mitophagy, autophagy, metabolism, and cellular senescence. MCL-1 is critical for embryonic development and associated with the survival of many cells, including the nervous system, T/B lymphocytes and cardiomyocytes [7].
This study revealed a complex and multifaceted nature of MCL-1 protein accumulation in B-cell malignancies upon treatment with MCL-1i (AMG-176 and AZD5991). They showed that the observed MCL-1 protein accumulation was unrelated to transcriptional activation of Mcl-1 gene but due to increased stability. However, this effect was reversible following withdrawal of MCL-1i, indicating a direct effect of the drug on MCL-1 protein stability. Using protein-protein interaction studies, immunoprecipitation (IP) and co-IP experiments, Tantawy et al. [14] showed that MCL-1i-induced defective ubiquitination of MCL-1 protein. This indicates that the upregulation of MCL-1 protein is not due to direct proteasomal inhibition, but rather due to interference with the ubiquitination and/or enhancing de-ubiquitination of MCL-1.
Tantawy et al. [14] further addressed the mechanisms underlying the decreased ubiquitination of MCL-1 protein and showed that MCL-1i increased MEK/ERK-mediated Thr 163 phosphorylation, leading to conformation change of MCL-1 protein. This in turn increases the surface accessible area to Thr 163 residue, thereby contributing to MCL-1 stability and accumulation. This observation was further supported by abolishing MCL-1 Thr 163 phosphorylation by using MCL-1-T163A phospho-mutant or direct inhibitor, trametinib, of upstream MEK/ERK pathway. In either approach, authors showed only partial effect of MCL-1i-induced reversal of MCL-1 protein upregulation in a cell type specific manner, suggesting the presence of other underlying mechanisms ( Figure 1A).
The group [14] further explored the effect of MCL-1i on the ubiquitination and de-ubiquitination of MCL-1. Using cell free in vitro ubiquitination/deubiquitination assays, the authors showed that MCL-1i directly enhanced DUB activity on MCL-1 protein, possibly by orienting MCL-1 to a state/conformation that does not favor ubiquitination and prefers deubiquitination by USP9x. This is further enhanced by the fact that MCL-1i disrupted MCL-1: Noxa interaction followed by rapid Noxa degradation and also associated with a transient decrease in the E3 ligase Mule protein level. Noxa normally degrades MCL-1 by favoring Mule-MCL-1 interaction and by opposing USP9x-MCL-1 interaction, thereby, its downregulation will contribute to MCL-1 protein stability. The contribution of DUBs in the observed MCL-1 stability was further re-affirmed by these authors using a global DUB inhibitor (WP1130), that rescued the MCL-1 upregulation induced by the MCL-1i ( Figure 1B). Interestingly, the two MCL-1i tested, AMG-176 and AZD5991, showed distinct effects on MCL-1 ubiquitination in a cell free in vitro ubiquitination assay, with AMG-176 enhancing while AZD5991 inhibiting it. Although the authors did not explore this unique observation further in detail, they predicted that it could be due to the binding difference between AMG-176 and AZD5991 to the BH3 binding grove of MCL-1 (AMG-176 lacks the salt bridge formation with Arg 263 of MCL-1) or due to different effect on the QRN motif of MCL-1 that may impact MCL-1 stability and degradation. Authors identified MCL-1i-induced important molecular changes particularly decrease in both Mule and Noxa protein levels, which may have implications in MCL-1i-induced cardiotoxicity. This is consistent with reports linking the critical role of Mule and Noxa in cardiotoxicity in murine models [15,16].
Despite high accumulation of MCL-1 protein after interaction with MCL-1i, there was induction of apoptosis. Authors explain this conundrum; MCL-1i disrupted both BAK and BAX interaction with MCL-1 which may be responsible for apoptosis ( Figure 1C). Interestingly, AZD5991 is more potent than AMG-176 in inducing apoptosis in either cell lines or in primary CLL lymphocytes, the reason for this difference is unknown.
Taken together, the study [14] provides novel insights into the regulation of MCL-1 expression by MCL-1i, associated molecular changes and their implications. They demonstrated that MCL-1i upregulated MCL-1 protein through direct and indirect mechanisms. MCL-1i led to enhanced DUB activity on MCL-1 protein, disruption and downregulation of Noxa as well as a transient decrease in Mule expression. The net effect was seen in MCL-1 protein stability. These molecular changes require further experiments to explore the potential role in MCL-1i-induced cardiotoxicity. Authors did not evaluate S63845 but identified differences between AMG-176 and AZD5991 in terms of potency. Collectively, these findings may have important implications for the development of next-generation MCL-1i with improved efficacy and safety profiles.

CONFLICTS OF INTEREST
Authors have no conflicts of interest to declare.