electrode and the working electrode create a potential difference in the solution, and a
current flows from the auxiliary electrode to the working electrode. In voltammetry, the
potential difference between the auxiliary and working electrodes is varied, and the current
between the two electrodes is examined. In impedance spectroscopy, the potential of the
working electrode is kept constant, and a sinusoidal voltage of fixed amplitude is applied to
the auxiliary electrode. The frequency of the sinusoidal signal is varied, and the output
signal frequency is examined rather than its amplitude. In potentiometric methods, the
electrochemical cell’s potential may be measured relative to a known reference potential,
with very little current flow. In amperometric methods, the intensity of the current flowing
through the electrochemical cell can be measured for a specific fixed potential.
An electrochemical biosensor consists of four functional components: an analyte, a
biorecognition element, a transducer, and an instrument. These components are needed,
independently of the method of analysis used. An analyte is a target of interest, such as a
protein or DNA. The biorecognition element is capable of selectively recognizing the
analyte. The transducer translates the interactions between the analyte and the bior
ecognition element into an electrical signal. A typical transducer for electrochemical
biosensors is an electrode that converts an ionic current into an electrical current or a
voltage, depending on the method used. The instrument usually consists of electronic
circuitry that captures, amplifies, and records biorecognition signals from the transducer.
The analyte is typically in a liquid medium that consists of an electrolyte solution that
maintains the analyte’s biological activity and transports it to the transducer.
6.3.2 Miniaturization of Electrochemical Biosensors and Example CMOS
Electrochemical Biosensors
The miniaturization of electrochemical biosensors is slated to increase their role in the
diagnosis of various diseases, particularly in resource-limited settings. There are two
main approaches towards the miniaturization of electrochemical biosensors. A note
worthy strategy is to use pre-existing hand-held instruments and modify them such that
they recognize biological components of interest that are different from those for which
they were originally intended. An example of such a biosensor is a glucometer that is
originally designed to detect blood glucose based on electrochemical signals generated by
redox reactions but that is retrofitted to recognize other analytes of interest. For instance,
the detection of non-glucose targets with a traditional miniaturized glucometer was
pioneered by Lu et al. [9]. They showed that by binding aptamers to targets with an
enzyme called invertase they could catalyze the hydrolysis of sucrose to glucose. Through
the generation of glucose catalyzed by invertase, a series of glucometer-based biosensors
were developed for a variety of analytical purposes such as the detection of disease
markers and the detection of DNA [10,11].
Another strategy, in scope with the present chapter, is to create miniature biosensor
systems based on CMOS sensors. Such an approach requires the integration of the in
strumentation circuitry and the biorecognition element on the same CMOS chip.
Furthermore, an often overlooked but necessary component is the hardware necessary for
delivering the analyte to the sensor sites. Such hardware typically includes microfluidic
networks, and their integration with CMOS chips has been covered extensively, for ex
ample by Huang et al. [12]. Below, we review a representative device that illustrates the
integration of electrochemical sensing into a CMOS platform.
The exemplary sensor was developed by Jafari et al. [13], and it was able to detect syn
thetic DNA sequences consistent with biomarkers for prostate cancer (Figure 6.3). Unlike
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