AI Article Synopsis

  • This paper introduces the first CMOS VEGF sensor designed for cancer diagnosis using human blood samples.
  • The sensor utilizes a peptide aptamer-based microneedle to detect electrochemical reactions with VEGF, subsequently read by a two-step capacitance-to-digital converter (CDC) that enhances measurement accuracy.
  • The prototype, built on a 65-nm CMOS process, exhibits low power consumption, high dynamic range, and impressive sensitivity in detecting VEGF, even in complex biological fluids like human blood serum.

Article Abstract

This paper presents the first CMOS Vascular Endothelial Growth Factor (VEGF) sensor for cancer diagnosis directly from human blood. The sensor incorporates a peptide aptamer-based microneedle that allows the detection of electrochemical reactions with VEGF. This results in a capacitance change between the microneedles and then reads out by a two-step capacitance-to-digital converter (CDC). The proposed two-step CDC consists of a coarse 5b slope ADC and a fine 14b continuous-time delta-sigma modulator (CTDSM). During slow peptide-binding, the slope ADC performs a coarse conversion and the results are used to adjust the current level of the stimulator. After settling of the peptide-binding, based on an adjusted stimulation current, the CTDSM measures the small capacitance changes of the sensor. The prototype chip is fabricated in a 65-nm CMOS process, occupying a 0.87 mm active area. The power consumption is 270 muW. Thanks to the two-step approach, this work achieves a wide dynamic range of 18.3b, covering a large sensor-to-sensor variation. It also achieves a peak resolution of 13.7b, while maintaining errors in 1 to 100 nF baseline capacitance. The overall sensor system successfully detects the VEGF in both phosphate-buffered saline (PBS) and human blood serum. Without the use of precision instruments, this work achieves a resolution of 15 fM [Formula: see text] in range of 0.1 to 1000 pM and denotes the clear VEGF selectivity at 40× in PBS and 5× in the blood serum compared to other proteins (IgG, Con A, and cholera toxin).

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Source
http://dx.doi.org/10.1109/TBCAS.2019.2954846DOI Listing

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