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Evaluation of Pyridaben Residues on Fruits Surface and its Stability by A Novel On-line Dual-frequency Ultrasonic Device and Chemiluminescence Detection Wangbing Zhang, Mei Wei, Wei Song, Yi-Xuan Gong, and Xin-An Yang J. Agric. Food Chem., Just Accepted Manuscript • DOI: 10.1021/acs.jafc.7b03357 • Publication Date (Web): 10 Oct 2017 Downloaded from http://pubs.acs.org on October 18, 2017
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Journal of Agricultural and Food Chemistry is published by the American Chemical Society. 1155 Sixteenth Street N.W., Washington, DC 20036 Published by American Chemical Society. Copyright © American Chemical Society. However, no copyright claim is made to original U.S. Government works, or works produced by employees of any Commonwealth realm Crown government in the course of their duties.
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Evaluation of Pyridaben Residues on Fruits Surface and
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its Stability by A Novel On-line Dual-frequency
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Ultrasonic Device and Chemiluminescence Detection Wang-Bing Zhang a*, Mei Wei a, Wei Song b, Yi-Xuan Gong a and Xin-An Yang a*
4 5
a
Department of Applied Chemistry, Anhui University of Technology, Maanshan, Anhui 243002, P. R.
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China b
Anhui Entry Exit Inspection and Quarantine Bureau, Hefei, Anhui 230022, P. R. China
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ABSTRACT: In this paper, we firstly report the development of a highly sensitive and economical
9
method for accurate analysis of pyridaben residues on fruits based on dual-frequency ultrasonic
10
treatment (DFUT) and flow injection chemiluminescence (CL) detection. The DFUT device is
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constituted
12
with different structures have been designed and applied to evaluate the function of DFUT in the
13
detection process. Recorded data showed that DFUT is an effective method for improving the pyridaben
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CL signal. The signal of pyridaben in response to DFUT is 2.0- 3.3 times stronger than the response to
15
only ultrasonic probe at 20kHz or ultrasonic bath at 40kHz, respectively. In addition, the response
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obtained from the concentric circles QGC is 2.1 times stronger than the response to the spiral tube QGC.
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Under the optimized condition, the proposed method has advantages, such as wide linear range
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(0.8-100.0 µg L-1), high sensitivity (limit of detection is 0.085 µg L-1) and good stability (RSDs ≤ 4.7%
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in the linear range) for pyridaben determination. We apply this method to monitor the residue pyridaben
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on some fruits. The data shows that the maximum amounts of residue on fruits surface after soaking in
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water (50 mg L-1, 5 min) are 0.583 mg kg-1 (apple), 0.794 mg kg-1 (orange) and 0.351 mg kg-1 (pear).
by integrating an ultrasonic bath with an ultrasonic probe. Two quartz glass coils (QGC)
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However, the concentration of pyridaben in presence of sunlight decreases rapidly, showing its poor
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light stability.
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Keyword: Dual-frequency ultrasonic irradiation; on-line CL determination; Pyridaben; Stability;
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Residue on fruits surface
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INTRODUCTION
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As
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4-chloropyridazin-3(2H)-one (Figure S1, Supporting Information), is widely used for controlling
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mites in fruit, tobacco, vegetable and other crops 1. Despite its low toxicity, overuse still can cause
30
harm to humans through food chain. For instance, Boyd et al. have reported that pyridaben can
31
affect the activity of mitochondrial complex I in the electron transport chain 2. Therefore, the
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maximum residue limits of pyridaben in some countries have been established, such as 0.5 mg kg-1
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in Spain (peppers, 7 day pre-harvest interval) 3, and 5 mg kg-1 in China (tea) 4.
one
of
the
nonsystemic
acaricide,
Pyridaben,
2-tert-butyl-5-(4-tert-butylbenzylehio)-
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Generally, chromatography with mass spectrometry or other selective and sensitive detectors is a
35
standard method for the determination of pyridaben. For example, Yang et al. reported a magnetic
36
mixed hemimicelles dispersive solid-phase extraction (MMHDSPE) with high performance liquid
37
chromatography (HPLC)-diode array method for determination of pyridaben in fruit juice 5. Sun et al.
38
developed a selective method for determination of pyridaben in citrus fruits by ultra-performance liquid
39
chromatography coupled with tandem mass spectrometry (UPLC–MS/MS), which limit of detection is l
40
µg kg-1 6. Douglas et al. established a sensitive procedure based on gas
41
triple-Quadrupole MS for pyridaben determination in several teas 7. Xiong et al. analyzed pyridaben in
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water and beverage samples by GC coupled with a flame photometric detector within a range of 8.0-600
43
µg L-1 8. Zhang et al. developed a protocol for the collection of LC electrospray ionization quadruple
44
linear ion trap MS for identification of pyridaben in peach 9. Frenich et al. proposed a method, in which
45
pressurized liquid extraction coupled with GS-MS/MS is used for identification of pyridaben in food
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commodities with limit of quantitation of 0.01 mg kg-1
10
chromatography
(GC)
. Liu et al. presented a quantification method
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based on HPLC-tandem MS for studying the dissipation of pyridaben in cabbage
. Many of these
48
above methods have excellent separation performance, which can analyze a large number of pesticide
49
residues in complex samples at the same time. However,
50
such separation and quantitative analysis,
comprehensive instruments are required in
thus high costs and other issues are particularly inevitable.
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Because of its easy operation, low cost and high sensitivity, chemiluminescence (CL) technique have
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been more and more used for pesticide residue detection in recent years. The analytes of this method
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including organophosphorus, organochlorines, and carbamate pesticide, and the limit of determination
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for each compound is lower than 0.01 mg L-1
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picoxystrobin, azoxystrobin, and fenpyroximate) determination, our studies indicate that direct detecting
56
by CL method is impossible, because these residues have no apparent effect on the traditional oxidant
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luminol CL systems (including luminol-H2O2, luminol-KMnO4, and luminol-K2S2O8, etc.). Subsequent
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experiments show that the CL intensity of these residues in luminol-oxidant system could be promoted
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in varying degrees after 10-30 min off-line ultrasonic bath treatment. And this enhancement is linearly
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related to the concentration of residues. The sensitivity and precision of the proposed method in our
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early works were superior or at least at the same level as those reported methods such as HPLC-MS and
62
GC-MS
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detection of pesticide residues is promising.
17-19
12-16
. For acaricide and fungicide residues (such as
, which indicated that the application prospect of ultrasonic assisted CL technology in the
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Compared with the previous work, the novelty of this study is to design a new dual-frequency
65
ultrasonic (DFUT) device, and build an on-line detection system with chemiluminescence detector, then
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solve the problems, such as loss of analyte, pollution and time-consuming during the off-line ultrasonic
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processing. Specifically, the ultrasonic device incorporating ultrasonic bath and ultrasonic probe, on one
68
hand, does not contact the sample solution directly during the process of ultrasonic irradiation, thus
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avoiding potential pollution problems. On the other hand, on-line processing and detection technology
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not only provides more rapid and real-time data acquisition, but also avoids the loss of the analyte. Also,
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the high ultrasonic densities of ultrasonic probe
20
coupled with the temperature control function of
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ultrasonic bath
may have higher efficiency for enhancing the response of chemiluminescence signal.
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The proposed on-line DFUT assisted CL method is used to evaluate pyridaben residues on fruits surface
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and its stability in sunlight. Its accuracy is confirmed by recovery experiments and HPLC-MS. As far as
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we know, no other study about the application of CL in the pyridaben monitoring had been reported.
76 77
Figure 1. Design of dual-frequency ultrasonic extraction scheme (a), a photo of QGC (b), and
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scheme of the FIA-CL system (c). QGC quartz glass coil; UBG ultrasonic bath generator; UPG
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ultrasonic probe generator; S sample; C acetonitrile solution (0.1% v/v); P1 P2 pump; V eight-port
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value; RC reaction cell; W waste; HV high voltage; PMT photomultiplier tube.
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EXPERIMENTAL PROCEDURES
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Apparatus and Materials. A homemade ultrasonic device (Figure 1A) is used to evaluate the
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efficiency of ultrasonic treatment. The device consists of an ultrasonic bath instrument
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(240mm×140mm×100mm) and an ultrasonic probe generator (20 kHz, Shanghai Guante Ultrasonic
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Instrument Co., Shanghai, China). Two quartz glass coils (QGC, 2mm i.d., 300mm length, ~ 920µL,
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Figure 1B) with different structures fixed on iron support as the reaction tubes are tested. Both ends
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of the QGC are made into elongated shape, to be easily connected to emulsion tube. The distance
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between QGC and the bottom of ultrasonic instrument (H1, cm) can be adjusted by changing the iron
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support height. The ultrasonic probe (8mm diameter, 150mm length) is positioned at a certain 4 Environment ACS Paragon Plus
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distance (H2, cm) above the QGC. The ultrasonic frequency of ultrasonic bath can be switched in
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three modes, 40, 50, 59 kHz. Besides, the temperature of water bath can be controlled by adjusting
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the flow rate of homemade external circulating water. Information about the CL detector, chemical
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reagents and sources used in the experiment are listed in Supporting Information.
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Sample Preparation. Fruit samples (apples, oranges, and pears) used in the experiment were
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purchased from local market. Before preparation, these samples are washed with double deionized
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water (DDW) and then air dried at 20oC. According to the literature
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follows. Firstly, nine samples including three apples (202.5g, 164.8g and 175.6g), three oranges
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(124.7g, 133.2g and 102.8g) and three pears (284.7g, 353.8g and 332.7g) are respectively dipped
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into beakers containing solution A (50.0 mg L-1 pyridaben, 300 mL) for 5 min and then the samples
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are taken out and air dried. Secondly, the dried samples are dipped into solution B (DDW, 300 mL)
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for 10 min and then the samples are taken out and air dried again. Thirdly, the dried samples are
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dipped into solution C (DDW, 200 mL) for 10 min.
13
, the samples are prepared as
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In order to know the change of pyridaben concentration in the above eluted solutions, 2.50 mL
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solution B and 10.00 mL C are quantitatively transferred into a 25mL colorimeter tube, respectively.
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And 2.50 mL acetonitrile-water solution (1% v/v) is added then dilute it to volume with DDW for
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CL determination.
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Analytical Procedures. The on-line DFUT and flow injection CL determination of samples are
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described in Figure 1C. Two peristaltic pumps named P1 and P2 are used to transport luminol and
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KMnO4 (P1), NaOH and pyridaben/carrier [acetonitrile-water (0.1% v/v)] solutions (P2) at the
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selected flow rate, respectively. Follow the experimental procedures listed in Table 1, the sample
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solution is firstly pumped from the colorimeter tubes to storage coil by P2 at a flow rate of 4.0 mL
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min-1. Next, the sample solution is driven into the QGC by the carrier at the same flow rate, where
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the sample is irradiated by selected ultrasonic conditions. The above solutions are mixed and reacted
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with luminol and KMnO4 in the reaction cell lastly, and the optical signal is recorded with the 5 Environment ACS Paragon Plus
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photomultiplier tube and the luminometer. Quantitative analysis is achieved by comparing the
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changes before and after the implementation of pyridaben. The calculation formula is ∆I=I-I0. I is
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the signal of pyridaben-luminol-KMnO4 system, and I0 is obtained under the same condition with
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acetonitrile-water (0.1% v/v) solution instead of pyridaben. Instrument settings and operational
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parameters of the experimental DFUT-CL system are summarized in Table S1 (Supporting
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Information).
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Table 1. Working program of the on-line ultrasonic treatment coupled with CL determination Flow rate/ mL min-1 Step
Time/s
Events
P1
P2
1
2.8
4.0
20
Draw sample solution through sampling tube
2
0.0
0.0
5
Move sampling tube into acetonitrile solution
3
2.8
4.0
20
Sample is carried into the QGC with acetonitrile solution
4
0.0
0.0
480 Sample is irradiated by ultrasound in the QGC
5
2.8
4.0
40
Reacting with luminol and KMnO4 , then record the CL signal
6
0.0
0.0
5
Return to step 1
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HPLC equipped with a ZORBAX XDB-C18 analytic column (2.1×150mm) and an MS detector
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(Agilent series 6430, USA), is used for recovery test to validate the accuracy and feasibility of the
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proposed method. Instrument settings and operational parameters used for the HPLC-MS system are
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summarized in Table S2 (Supporting Information).
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RESULTS AND DISCUSSION
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DFUT-CL Determination of Pyridaben. In general, the quantitative basis of the CL method is that
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the analyte improves or inhibits the optical signal of different luminescence system 6 Environment ACS Paragon Plus
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. However,
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preliminary experimental data shows that the addition of pyridaben doesn't change the CL signals of
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luminol with H2O2, KMnO4 or K2S2O8. When the on-line DFUT procedure is carried out before the
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pyridaben mixing with oxidant and luminol, fortunately, the CL signal of the luminol-oxidant
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system is markedly enhanced. Figure 2 shows the effect of different concentration of pyridaben on
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the CL signal in the luminol-KMnO4 system after DFUT. A good linear relationship (R2=0.9985)
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between the relative CL signal (∆I) and pyridaben concentration (inset of Figure 2) range from 0.8
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to 100.0 µg L-1 displays the wide linear range of the proposed methods in the field of monitoring
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pyridaben.
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Figure 2. CL intensities of different concentration of pyridaben after on-line DFUT (For the
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convenience of description, the time required for ultrasonic treatment in each measurement process
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is subtracted). Conditions of DFUT: 20kHz ultrasonic probe + 59kHz ultrasonic bath (frequency),
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20W + 80 W (power), 50oC (temperature), 6min (time).
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The mechanism of the enhancing effect on the CL signal is considered as a kind of energy transfer
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process based on the following experimental facts: i) there is no difference in HPLC-MS
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chromagraphy between before and after ultrasonic treatment (Figure S2, Supporting Information),
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which indicates that ultrasound does not promote degradation of pyridaben. ii) Except for peak
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intensity change,there is no new peak is found in the fluorescence and UV spectra of the 7 Environment ACS Paragon Plus
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luminol-KMnO4-pyridaben with/without DFUT (Figure S3, Supporting Information), which confirm
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that the emission spectrum belongs to 3-aminophthalate ion (3-AP). iii) the enhancement of CL
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signal is linearly related to the concentration of pyridaben, showing that pyridaben is involved in the
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luminescence process, not just because of hydroxyl radical produced in ultrasound.
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Figure 3. Diagram of the mechanism. We present the reaction process depicted in Figure 3. Briefly, under the irradiation of ultrasound, 22, 23
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water molecules produce hydroxyl radical (·OH) with high activity
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pyridaben gaining higher energy (excited). When the excited state of aminophthalate (3-AP*,
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produced by reaction between luminol and KMnO4) releases energy from the excited state back to
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the ground state, it can obtain energy from excited pyridaben molecules and re-excited to 3-AP*.
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Obviously, CL intensity is enhanced in the above process 24. More detailed explanations are listed in
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the Supporting Information.
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Optimum of Ultrasonic Conditions. Effect of ultrasonic mode on the signal of pyridaben. Based on
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the frequency and number of ultrasonic waves applied, we tested the effect of pyridaben on the CL
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signals of the luminol-KMnO4 system in seven ultrasonic modes after 10 min irradiation. The results
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are shown in Figure 4, the highest CL signal is obtained in the 20kHz ultrasonic probe + 59kHz 8 Environment ACS Paragon Plus
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ultrasonic bath mode. Compared with this mode, the CL signals of pyridaben irradiated by 20kHz
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ultrasonic probe and 59kHz ultrasonic bath separately are about 50% and 30%, respectively.
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Figure 4. Effect of ultrasonic mode on the CL intensities. Conditions of ultrasonic treatment are listed in
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Table 1. UB ultrasonic bath; UP ultrasonic probe.
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Gogate pointed out that the cavitation bubbles produced by high frequency ultrasonic wave can be 25
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used as the nuclei of lower frequency cavitation
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dual-frequency ultrasound is quite different from that of single frequency 26, 27. And these cavitation
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bubbles lead to more homogeneous and intense cavitation effect as compared to a single frequency
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sounding
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formation of hydroxyl radicals (·OH). Besides, an interesting experimental phenomenon either
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dual-frequency mode or single-frequency mode is found, that the increase of the CL signal is related
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to the applied ultrasonic frequency. The CL signals of pyridaben in Figure 4 are increased about
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30% (dual-frequency mode) and 22% (single-frequency mode) with the UB frequency from 40kHz
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to 59kHz. As we know, the cavitation effect is related to the size of the resonant bubble radius (r)
179
and bubble collapse time (τ). Although small bubbles produce weak cavitation 30, a decrease of more
28, 29
. Therefore, the size of cavitation bubbles in
. This high intensity cavitation effect under dual-frequency mode promotes the
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than 40% in collapse time (Table S3, Supporting Information) give rise to more acoustic cycles and
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results in the formation of large amounts of smaller sizes cavitations bubbles at higher frequencies,
182
and thus more cavitations per unit time
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production, thus promote pyridaben to form excited products.
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Effect of QGC shape and position.Two shapes of QGC are applied to the ultrasonic irradiation of
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pyridaben (Figure 1B). One of the QGC is concentric circles shape, and the other one is a spiral
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tube. The position of QGC in the ultrasonic device is also important in the process of ultrasonic
187
irradiation
188
considered together in this paper.
32
31
. Obviously, these factors are beneficial to radical
. Therefore, the effects of QGC shape and position on the signal intensity of CL are
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Figure 5 displays the signal change tendency after changing the position of QGC in the device. This
190
experiment is carried out by fixing one of distance (H1 or H2) at 1.0 cm. Figure 5A indicates that the CL
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signal intensity decreases remarkably both with the distance of H1 and H2 from 0.5 to 4.0cm for 20 µg
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L-1 pyridaben solution when the threaded tubes QGC is used. Figure 5B indicates that the CL signal
193
intensity increases both with the distance of H1 and H2 from 0.5 to 1.0cm, and then rapidly decreases
194
when the concentric circle QGC is used. Compared with the distance between QGC and bottom of
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ultrasonic bath (H1), the change of ultrasonic probe position (H2) caused more severe signal changes,
196
which indicated that the distance has more influence on ultrasonic probe.
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Figure 5 also shows that the shape of QGC is an important factor that impacts signal intensity. Under
198
the same conditions, the response obtained from the concentric circles QGC is 2.1 time of that from the
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spiral tube QGC. The reason may be that the size (2.0 cm) of the spiral tube caused the solution in the
200
tube to be farther away from the probe than the solution in the concentric circles QGC. Therefore, the
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concentric circles QGC placed at the middle of the two ultrasonic devices (H1= H2 = 1.0 cm) is used as
202
the optimum conditions in the sample analysis process with the best stability. Meanwhile, RSDs of 11
203
times measurements are less than 4.7% within linear range (e.g. 1.3% for 20µg L-1 and 2.5% for 50µg
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L-1, Figure S4, Supporting Information). Also, good stability of the proposed methods is documented. 10 Environment ACS Paragon Plus
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Figure 5. Effect of QGC shape and position on the CL intensity of 20 µg L-1 pyridaben. (a) for spiral
207
tube shape, and (b) for concentric circles shape. H1 (H2) is optimized by fixing the distance of H2 (H1) at
208
1cm.
209 210
Figure 6. Effect of time on the CL intensities. Conditions of ultrasonic treatment were listed in Table S1.
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UB ultrasonic bath ; UP ultrasonic probe.
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Effect of Ultrasonic Time. Figure 6 lists the change of the CL signal of pyridaben-luminol-KMnO4
213
with different ultrasonic time. The relative signal of the luminol-KMnO4 system increases with the
214
increased residence time for pyridaben sample solution stay in the QGC, and reaches the maximum 11 Environment ACS Paragon Plus
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signal at 8min (20kHz UP + 59kHz UB), 22min (20kHz UP) and 40min (59kHz UB), respectively.
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Then the signal decreases with the prolonging of time. In addition, the maximum CL signals
217
obtained under the three modes are also different. As can be seen in Figure 6, the relative CL signals
218
of the pyridaben-luminol-KMnO4 system are only 73% (20kHz UP) and 61% (59kHz UB) of that
219
irradiated by dual-frequency mode with the same concentration.
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Moreover, in a dual-frequency ultrasonic mode, the higher ultrasonic frequency, the shorter the
221
time required to reach maximum signal. For instance, when the 20kHz UP + 59kHz UB
222
dual-frequency mode is applied, it’s need 8 min to reach the maximum. When the 20kHz UP +
223
40kHz UB mode is used, the time is increased to 12 min (data not shown here). Meanwhile, the
224
signals of pyridaben are decreased after ultrasonic treatment for a long time. It’s shows that
225
prolonging the ultrasonic time does not yield stronger signal. It should be noted that the appropriate
226
response signal can also be obtained by shortening the ultrasonic processing time to 3-4min.
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Effect of Ultrasonic Power and Temperature. The effect of ultrasonic power on the CL signal in the
228
pyridaben-luminol-KMnO4 system is studied by fixed the ultrasonic probe power at 80 W. Figure
229
S5A-C (Supporting Information) shows the changes in the relative CL signals of the
230
pyridaben-luminol-KMnO4 system produced by varying the power of the ultrasonic bath under different
231
dual-frequency modes. Due to violent cavitation at high ultrasonic power, the acoustic reaction of H2O
232
is accelerated 32, resulting in linear enhancement of the relative CL signal of pyridaben-luminol-KMnO4
233
with ultrasonic power (Figure S5D, Supporting Information). As a result, 200W (the maximum power
234
of the ultrasonic bath) is selected.
235
The influence of bath temperature is investigated by the temperature control function of ultrasonic
236
bath. The results are shown in Figure S6 (Supporting Information). When the temperature reaches 50oC,
237
the DUFT-CL signal of pyridaben is the highest. The influence of temperature on the CL signal is
238
basically independent of the applied ultrasonic frequency (Figure S6D, Supporting Information).
239
Although more cavitation bubbles formed in high temperatures
30-32
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weakened when the temperature is too high (e.g. up to 70 oC in our experiment). Therefore, 50 oC is a
241
better temperature.
242
Optimization of CL Conditions. In general, the higher luminol concentration, the larger CL signal will
243
be obtained
244
intensity increases with the increase of the luminol concentration in the range of 1.0×10-5mol L-1 to
245
1.0×10-4 mol L-1. As the concentration exceeds 7.0×10-5 mol L-1, the upward tendency of the signal
246
becomes slighter. These data can be found in Figure S7A (Supporting Information). CL reaction usually
247
is not complete at low KMnO4 concentration, and the self-absorption effect of KMnO4 at high
248
concentration will also affect the sensitivity of the method
249
result (Figure S7B, Supporting Information). Therefore, 5.0×10-5 mol L-1 KMnO4 based on the
250
experimental data is selected as the operating condition. The luminol-KMnO4 reaction usually takes
251
place in an alkaline medium. The biggest CL signal of the pyriden-luminol-KMnO4 system in our
252
experiment is obtained at NaOH concentration range from 0.6 to 1.0 mol L-1 (Figure S7C, Supporting
253
Information). Two peristaltic pumps are used to transport the reactants in this experiment, thus the flow
254
rate not only affects the degree of CL reaction but also causes the waste of reagents 19. When the flow
255
rate of two peristaltic pumps are set at 2.8 mL min-1 (P1, luminol, and KMnO4) and 4.0 ml min-1 (P2,
256
NaOH, and analytes), respectively, the relative CL signal are suitable (Figure S8, Supporting
257
Information).
258
Interference Study. The effect of the presence of foreign substances in solution, on pyridaben
259
determination by CL with ultrasonic assistance, is tested. The tolerable concentration ratios with respect
260
to 2.0 µg L-1 pyridaben for interference at 5% level are over 10,000 for Na+, K+, Ca2+, Mn2+, Cl-, SO42-,
261
CO32-, NO3- and H2PO4-; 2000 for Ba2+, Mg2+, Al3+ and Zn2+; 500 for methanol, ethanol, oxalate, tartrate,
262
urea; 100 for ascorbic acid, L-cysteine, Cu2+, Fe3+, Cr3+, Co2+ and Ni2+. The detailed results are listed in
263
Table 2.
264
Table 2. Effect of coexisting substances on the determination of 2.0 µg L-1pyridaben.
15-18
. Our experimental data also confirms this conclusion. Although, briefly, the CL
17
. The experimental data show a similar
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Species Cu2+
Co2+
Fe3+
Ni2+
Cr3+ Na+ K+ Ca2+ Ba2+ Mg2+ Al3+
C, mg L-1 Recovery, % 0.1 101 0.2 105 1.0 121 0.1 97 0.2 95 1.0 118 0.1 99 0.2 104 1.0 112 0.1 97 0.2 102 1.0 106 0.1 105 0.2 104 1.0 107 20 96 20 97 20 97 4 98 4 102 4 104
Species methanol oxalate ethanol tartrate urea ascorbic acid L-cysteine
ClNO3H2PO4CO32SO42HPO42-
C, mg L-1 1.0 5.0 1.0 5.0 1.0 5.0 1.0 5.0 1.0 5.0 0.2 0.5 0.1 0.2 1.0 20 20 20 20 20 20
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Recovery, % 98 92 103 94 97 90 95 91 102 94 96 87 102 95 81 101 99 104 98 97 105
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The mechanism of the enhancing effect on the CL signal is considered as a kind of energy transfer
266
process. Hence, some agrochemicals may also enhance the luminescence signal of lumilo-oxidant after
267
ultrasonic treatment. Experimental data show that the presence of 10.0 µg L-1 substances in 2.0 µg L-1
268
pyridaben sample solution produce 35% (picoxystrobin), 43% (azoxystrobin) and 27% (fenpyroximate)
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positive interference; 20.0 µg L-1 substances in 2.0 µg L-1 pyridaben can lead to 52% (picoxystrobin),
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69% (azoxystrobin) and 58% (fenpyroximate) changes. Besides, the CL detector itself does not have
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selective analysis function. These factors will lead to problems, that is the presented method can not be
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used directly for complex sample analysis. We are seeking for suitable ways (e.g. combination with
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chromatographic separation or selective extraction for multiple-residues samples analysis) to resolve
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this problem.
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Performance and Validation of the Procedure. Under the selective conditions, linear revision
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diagram is available in the scale of 0.8-100.0µg L-1 with the linear regression equations: IF=57.67 +
14 Environment ACS Paragon Plus
Page 15 of 30
Journal of Agricultural and Food Chemistry
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214.03 C. C in the equation is the pyridaben concentration (µg L-1). The regression coefficient (r2) is
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0.9974. The limit of detection (LOD) of pyridaben for this method is 0.085 µg L-1, calculated by taking
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3 times the standard deviation of the blank solution divided by the slope from 11 measurements. The
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limit of quantitation is 0.284 µg L-1. An analytic frequency of 6 h-1 (or 15 h-1 with 3min DFUT and the
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LOQ is 1.025 µg L-1) and an RSD value of 1.3% (at the 20.0 µg L-1 level for eleven replicate
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determinations) are also obtained. Table 3 covers the merits of analytical data achieved by using on-line
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DFUT coupled with CL for sample detection and the comparison of analytical performance with several
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other methods are also listed. The sensitivity and precision are superior or at least at the same level as
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reported methodologies.
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Table 3. Comparison of analytical parameters with other methods. Analytical Method
Linear range, µg L-1
LOD, µg L-1
RSD, %
Ref.
DFUT-CL a
0.8-100.0
0.085
