AI Article Synopsis

  • Estrogen receptor α (ERα) is a key biomarker in breast cancer that influences diagnosis and treatment strategies, making its accurate detection vital for patient outcomes.
  • A new liquid-gated graphene field-effect transistor (FET) biosensor was developed for quick and label-free detection of ERα, utilizing a specially synthesized drug molecule as a capture probe.
  • The sensor demonstrated high sensitivity with a low detection limit (2.62 fM) and could effectively differentiate between ERα-positive and ERα-negative samples from 36 cell lysates within 30 minutes, highlighting its potential for rapid breast cancer diagnostics.

Article Abstract

Estrogen receptor α (ERα) is an important biomarker in breast cancer diagnosis and treatment. Sensitive and accurate detection of ERα protein expression is crucial in guiding selection of an appropriate therapeutic strategy to improve the effectiveness and prognosis of breast cancer treatment. Herein, we report a liquid-gated graphene field-effect transistor (FET) biosensor that enables rapid, sensitive, and label-free detection of the ERα protein by employing a novel drug molecule as a capture probe. The drug molecule was synthesized and subsequently immobilized onto the sensing surface of the fabricated graphene FET, which was able to distinguish the ERα-positive from the ERα-negative protein. The developed sensor not only demonstrated a low detection limit (LOD: 2.62 fM) but also achieved a fast response to ERα protein samples within 30 min. Moreover, depending on the relationship between the change of dirac point and the ERα protein concentrations, the dissociation constant () was estimated to be 7.35 ± 0.06 pM, indicating that the drug probe-modified graphene FET had a good affinity with ERα protein. The nanosensor was able to analyze ERα proteins from 36 cell samples lysates. These results show that the graphene FET sensor was able to differentiate between ERα-positive and ERα-negative cells, indicating a promising biosensor for the ultrasensitive and rapid detection of ERα protein without antibody labeling.

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Source
http://dx.doi.org/10.1021/acs.analchem.3c04809DOI Listing

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