Pharmacogenomic and Circulating Biomarkers for CDK4/6 Inhibitors

Pharmacogenomic and Circulating Biomarkers for Predicting Toxicity or Suboptimal Benefit From Small Molecule Kinase Inhibitor Therapy

Status

Enrolling by invitation

Phases

Unknown

Study type

Observational

Source

ClinicalTrials.gov

Registry ID

NCT07100054

Enrollment

100

Registered

2025-08-01

Start date

2025-10-10

Completion date

2028-09-30

Last updated

2025-12-12

For informational purposes only — not medical advice. Sourced from public registries and may not reflect the latest updates. Terms

Conditions

CDK4/6 Inhibitor, Breast Cancer, CYP3A4 Protein, Human, Drug Interaction, Pharmacogenetic Testing

Brief summary

The goal of this research study is to reduce adverse effects of anti-cancer medications known as kinase inhibitors, while preserving their therapeutic benefits. There have been major advances in the way cancers are treated. A class of drugs known as kinase inhibitors have proven to be highly effective for the treatment of cancers, including lung, kidney, gastrointestinal, and breast cancers. However, kinase inhibitor medications are well known for having unpredictable side effects. The body breaks down (metabolizes) medications such as kinase inhibitors using an enzyme known as cytochrome P450 3A4 (CYP3A4). CYP3A4 is the most important drug metabolizing enzyme in humans due to the fact that it is involved in the metabolism of nearly half of all prescribed medications and almost all of the currently prescribed kinase inhibitors. Among patients, there can be nearly 400 times difference in how efficiently CYP3A4 metabolizes drugs. Remarkably, very little is known about the role of genetic differences in CYP3A4 and a gene known as pregnane X receptor (PXR). PXR serves as a sensor for drugs in the body and helps to regulate how much CYP3A4 is made. Currently, there are no predictive biomarkers, whether in genes (genomic) or circulating in blood (endogenous) that could aid treating oncologists with regards predicting adverse effects or suboptimal response to this important class of anticancer drugs. The goal is to carry out DNA sequencing for genetic changes in CYP3A4 and PXR to assess differences in enzyme activity of not only common, but also rare genetic variants. CYP3A4 activity will be determined in participants blood samples based on break down products of the drug tamoxifen as well as cholesterol, the latter called 4β-hydroxycholesterol, both known to be influenced by the CYP3A4 enzyme. Since cholesterol is naturally made in the body, comparing blood cholesterol to 4β-hydroxycholesterol levels will be a biomarker of CYP3A4 metabolic activity that can be measured in anyone. Furthermore, circulating CYP3A4 messenger RNA from human blood will be measured as another independent marker of CYP3A4 gene expression. A model will be generated that includes these biomarkers of CYP3A4 expression and function, as well as genetic variation in CYP3A4 and PXR, that will aid in better identifying which patients may be at risk for loss of benefit or toxicity from kinase inhibitor therapy. This model will be evaluated in 100 breast cancer patients undergoing chemotherapy with kinase inhibitors, namely cyclin-dependent kinases CDK4 and CDK6 inhibitor (abemaciclib, ribociclib or palbociclib), as such kinase inhibitors are widely prescribed for breast cancer and are known to be broken down by CYP3A4.

Interventions

GENETICWhole gene sequencing

Whole gene sequencing of CYP3A4 and PXR

OTHERDrug-drug interaction analysis

Evaluating potential drug interactions with CYP3A4 inhibitors and inducers

OTHERBiomarker analysis

Determination of circulating CYP3A4 mRNA, and 4b-hydroxycholesterol

Study design

Observational model

COHORT

Time perspective

PROSPECTIVE

Eligibility

Sex/Gender

FEMALE

Age

18 Years to No maximum

Healthy volunteers

Inclusion criteria

* female * breast cancer diagnosis * over 18 years of age * indication for a CDK4/6 inhibitor treatment * proficient in English

Exclusion criteria

* None

Design outcomes

Primary

Measure	Time frame	Description
Predictive model for CDK4/6 inhibitor concentrations	From enrollment to 3 months	A linear mixed effect model will be applied using CDK4/6 inhibitor levels considering the following independent variables: sex, age, body surface area, height, weight, serum creatinine, drug dose, CYP3A4 and PXR genotype (any impaired-function SNV carrier vs. normal function SNV carrier status/wildtype as per in vitro analysis), CYP3A4 mRNA and 4β-hydroxycholesterol. The model that best describes the fit of CDK4/6 pharmacokinetics will be selected.

Secondary

Measure	Time frame	Description
Patient reported outcomes	From enrollment to 3 months	Evaluate the association in patient reported outcomes in the EORTC QLG Core Questionnaire (EORTC QLC-C30) with drug concentrations and/or treatment-related toxicity using common terminology criteria for adverse events (CTCAE). CTCAE is graded on a scale from 1 to 5 with a higher number indicating more toxicity. The EORTC QLC-C30 is a 30-item instrument to assess quality of life. The first 28 items are rated on a scale from 1 to 4 with a higher score indicating worse outcome. The last 2 items are rated on a scale of 1 to 7 with a higher number indicating better health and quality of life.

Other

Measure	Time frame	Description
Exploratory breast cancer outcomes	From enrollment to 3 months	Evaluate efficacy of CDK4/6 by examining breast cancer outcomes, including invasive disease-free survival (IDFS) and overall survival (OS)

Countries

Canada

Outcome results

None listed

Source: ClinicalTrials.gov · Data processed: Feb 4, 2026