| Literature DB >> 26885393 |
Kusum Lata1, Vikas Dhull2, Vikas Hooda1.
Abstract
The developed method used three enzymes comprised of cholesterol esterase, cholesterol oxidase, and peroxidase for fabrication of amperometric biosensor in order to determine total cholesterol in serum samples. Gold nanoparticles (AuNPs) and carboxylated multiwall carbon nanotubes (cMWCNTs) were used to design core of working electrode, having covalently immobilized ChO, ChE, and HRP. Polyacrylamide layer was finally coated on working electrode in order to prevent enzyme leaching. Chemically synthesised Au nanoparticles were subjected to transmission electron microscopy (TEM) for analysing the shape and size of the particles. Working electrode was subjected to FTIR and XRD. The combined action of AuNP and c-MWCNT showed enhancement in electrocatalytic activity at a very low potential of 0.27 V. The pH 7, temperature 40°C, and response time of 20 seconds, respectively, were observed. The biosensor shows a broad linear range from 0.5 mg/dL to 250 mg/dL (0.01 mM-5.83 mM) with minimum detection limit being 0.5 mg/dL (0.01 mM). The biosensor showed reusability of more than 45 times and was stable for 60 days. The biosensor was successfully tested for determining total cholesterol in serum samples amperometrically with no significant interference by serum components.Entities:
Year: 2016 PMID: 26885393 PMCID: PMC4739480 DOI: 10.1155/2016/1545206
Source DB: PubMed Journal: Biochem Res Int
Figure 1Transmission electron microscopy (TEM) of gold nanoparticles. (a) Aggregates of gold nanoparticles, (b) dimensions of a tuft of nanoparticles, and (c) enlarged image for size analysis.
Figure 2X-ray diffraction patterns of c-MWCNTs (a) and AuNP/c-MWCNTs (b).
Figure 3SEM images of (a) electrode without enzyme and (b) with enzyme.
Figure 4Cyclic voltammogram of ChE/ChO/HRP-AuNPs/c-MWCNTs Ag electrode at various scan rates.
Figure 5Cyclic voltammogram. (A) ChE/ChO/HRP-AuNPs/c-MWCNTs; (B) bare silver electrode.
Figure 6Response of current with applied potential.
Figure 7Effect of pH on current response of the present method.
Figure 8Effect of incubation temperature on the response of present method.
Figure 9Response time of the current method.
Figure 10Effect of cholesteryl acetate concentration on the present method.
Figure 11Lineweaver-Burk plot of the present method.
Analytical recovery calculated by using added cholesteryl acetate in serum sample.
| Cholesteryl acetate added (mg/dL) | Cholesteryl acetate found (mg/dL) | % recovery | S.D. |
|---|---|---|---|
| Nil | 173.74 | — | — |
| 100 | 271.33 | 99.11 | 0.88 |
| 200 | 368.79 | 98.67 | 0.93 |
Within batch and between batches coefficients of variation for determination of total cholesterol in serum samples.
|
| Total cholesterol (mg/dL) | CV (%) |
|---|---|---|
| Within batch (6) | 170.02 ± 1.04 | 0.61 |
| Between batches (6) | 169.96 ± 1.6 | 0.98 |
Comparison of the present method with previously reported biosensor for total cholesterol determination.
| Transducer | Method of enzyme immobilization | Working potential | Response time | Detection limit | Linearity | Storage stability | Reference |
|---|---|---|---|---|---|---|---|
| Laponite clay nanoparticles-pol((12-pyrrol-1-dodecyl)triethylammonium tetrafluoroborate)/Pt disk electrode | ChO, ChE enzyme Entrapment | 0.53 V versus Ag/AgCl | 50 sec | 20 | — | 20 days | [ |
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| Screen printed graphite electrode | ChO, ChE, HRP, K4Fe(CN)6 | −0.2 V versus Ag/AgCl | — | 2.81 mM | 2.81–13 mM | — | [ |
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| Polydiaminonaphthalene/Pt disk | ChO, ChE | 0.7 V versus Ag/AgCl | 15 sec | 97 | Up to 0.8 mM | — | [ |
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| MWCN/screen printed carbon electrode | ChO, ChE, HRP, K4Fe(CN)6 | 0.3 V versus Ag/AgCl | 180 sec | 100 mg/dL | 100–400 mg/dL | 2 months |
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| 3-Aminopropyl-modified controlled-pore glass(APCEG)/rotating disk | ChO, ChE, HRP | −0.15 V versus Ag/AgCl with TBC as mediator | — | 11.9 nM | 1.2 | 25 days | [ |
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| PANI/ITO | ChO, ChE | 0.5 V versus Ag/AgCl | 40 sec | 50 mg/dL | 50–500 mg/dL | 6 weeks | [ |
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| HRP incorporated carbon paste | ChO, ChE | −0.5 V versus Ag/AgCl | 20 sec | 2.5 mg/dL | 50–550 mg/dL | 100 days | [ |
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| Nanoporous Au networks directly grown on a titanium substrate | ChO, ChE, HRP | Cyclic voltammetry | — | 0.5 mg/dL | 0.97–7.8 mM | 60 days | [ |
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| ZnO–CuO composite matrix grown onto ITO coated corning glass | ChO, ChE | Cyclic voltammetry | 5 sec | 0.5 mM | 0.5–12 mM | — | [ |
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| c-MWCNT/AuNP | ChO, ChE, HRP | 0.27 V versus Ag/AgCl | 20 sec | 0.5 mg/dL | 0.5–300 mg/dL | 60 days | This work |
Figure 12Correlation between cholesteryl acetate concentrations in serum determined by standard enzo kit method (x-axis) and by the present method (y-axis).
Effect of different serum substances on the working of CH biosensor.
| Compounds added | Final conc. (physiological conc.) (g/L) | % relative response |
|---|---|---|
| None | — | 100 |
| Glucose | 0.90 | 99 |
| Uric acid | 0.03 | 100 |
| Ascorbic acid | <17 | 101 |
| Urea | 0.10 | 98 |
| Ca2+ | 11.5 | 99 |
| Acetone | 0.02 | 98 |
| Bilirubin | 2.2 | 100 |
Figure 13Reusability of the present method.
Figure 14Storage stability of the present method.
Total cholesterol level in serum of probably healthy individuals calculated by current biosensor.
| Age group | Sex | Total cholesterol in serum mg/dL |
|---|---|---|
| <10 | M | 154.17 ± 2.04 |
| F | 144.56 ± 3.05 | |
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| 11–20 | M | 170.14 ± 6.57 |
| F | 163.95 ± 4.31 | |
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| 21–30 | M | 189.24 ± 5.45 |
| F | 185.64 ± 6.08 | |
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| 31–40 | M | 199.87 ± 7.01 |
| F | 190.02 ± 9.02 | |
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| 41–50 | M | 208.56 ± 8.18 |
| F | 195.72 ± 8.16 | |
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| 51–60 | M | 223.56 ± 6.02 |
| F | 217.34 ± 5.06 | |
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| 61 & above | M | 225.89 ± 6.05 |
| F | 225.58 ± 9.03 | |
Working parameters of the newly developed method.
| Parameters | Present method |
|---|---|
| pH | 7 |
| Temperature (°C) | 40 |
| Working potential (V) | +0.27 |
|
| 58.7 (1.36 mM) |
|
| 0.9 |
| Detection limit (mg/dL) | 0.5 (0.01 mM) |
| Linearity (mg/dL) | 0.5–250 (0.01 mM–5.8 mM) |
| Response time (sec) | 20 |
| Storage stability (days) | 60 |