Synthesis of Dacus Pheromone, 1,7-Dioxaspiro[5.5]Undecane and Its Encapsulation in PLLA Microspheres for Their Potential Use as Controlled Release Devices

Olive fruit fly Dacus oleae is a well-known pest infecting the bark of olive fruit, leading to reduction of extracted olive oil properties. Among chemicals proposed for Dacus oleae population control, pheromone 1,7-dioxaspiro(5.5)undecane (DSU), Dacus pheromone, is considered as a promising agent, which is added in several traps. However, all proposed systems manage to sufficiently deliver DSU for only two weeks. Furthermore, an additional problem is the limited available amount of pheromone to use in such systems. To overcome this, in the present study, a novel synthetic procedure of DSU is described, including only five steps. Intermediate products were studied by High Resolution Mass Spectroscopy Electrospray Ionization (HRMS-ESI) (m/z), while the resulting DSU was further characterized by 1H and 13C-NMR. Synthesized DSU was further encapsulated in poly(L-lactic acid) (PLLA) microparticles in three different concentrations; 5, 10 and 20% w/w. Its successful incorporation was studied by FT-IR, XRD and differential scanning calorimeter (DSC) while two procedures, liquid extraction and solid phase microextraction, followed by GC-MS analysis, was used for quantification of pheromone to microparticles. It was found that microparticles loading was over 85% for all three formulations. Its release showed a prolonged profile for microparticles containing 20% w/w DSU, lasting four weeks, while the quantity of DSU released reached 100%. These microparticles could be appropriate to control Dacus oleae population.


Introduction
Olive oil is considered to be the "green gold" of the Mediterranean Region where Olea europaea L. is thriving. Spain, Italy and Greece are the three countries associating with the main production of olive oil and in the resent years, countries of northern Africa, such as Algeria are trying to take part in international production. Olive oil owes its benefits to its properties; i.e., high phenolic compounds leading to antioxidant and antibacterial properties. Hence, these properties are found to be reduced resources such as potato, corn, cane molasses and beet sugar, while its bioabsorbable character and its promising mechanical properties surely make it an attractive and useful biodegradable polymer with a wide range of applications [15]. PLA is mainly used in biomedical application and drug delivery systems [16][17][18][19] in the form of micro-and nanoparticles [20,21]. The advantage of these systems is that the active compound is homogeneously encapsulated in PLA particles and the release of them can last for many days. This is also the main target of the present work. To develop of a new approach for DSU synthesis and its further encapsulation in PLLA microspheres for their potential use as suitable polymer carriers for subsequent controlled release of DSU over an extended period. As far as of our knowledge analogous study for encapsulation of Dacus pheromone has not been conducted before.

Preparation of PLLA Microparticles
Polymeric microspheres containing 1,7-dioxaspiro [5.5]undecane were prepared by oil-water (o/w) emulsification method, as was previously reported by Nanaki et al. [16,19,25]. In brief, PLLA was dissolved in 5 mL dichloromethane and 1,7-dioxaspiro [5.5]undecane was inserted in the polymeric solution in ratios 5, 10 and 20% w/w followed by probe sonicator for 1 min, cycle 1, amplitude 100% (UP50H, Hielscher Ultrasound Technology, Teltow, Germany). The dispersion was added dropwise in 20 mL of PVA solution, 1% w/v concentration, and homogenized at 30,000 rpm for 1 min (T 10 basic Ultra-Turrax, IKA, Staufen im Breisgau, Germany). After that, it was added to 20 mL H 2 O and left under magnetic stirring till total evaporation of dichloromethane. After centrifugation at 9000 rpm for 20 min (Heraeus™ Pico™ 17 Microcentrifuge, Thermo Fisher Scientific, Waltham, MA, USA) the resulting microparticles were washed with distilled water in order to remove the residual PVA and freeze-dried. Net microparticles of PLLA were also prepared by the same procedure for comparison reasons.

Characterization of Prepared Microspheres
Thermogravimetric Analysis (TGA) Thermogravimetric analysis was carried out with a SETARAM SETSYS TG-DTA 16/18. Samples (6.0 ± 0.2 mg) were placed in alumina crucibles. An empty alumina crucible was used as reference. PLLA and PLLA-DSU microparticles were heated from ambient temperature to 700 • C in a 50 mL/min flow of N 2 at heating rate of 20 • C/min. Continuous recordings of sample temperature, sample weight, its first derivative and heat flow were performed.
Fourier Transform-Infrared Spectroscopy (FT-IR) The chemical structure of the synthesized materials was determined with the use of FTIR spectroscopy. FTIR spectra of the samples were received with an FTIR spectrometer (model FTIR-2000, Perkin Elmer) using KBr discs (thickness of 500 µm). Infrared (IR) absorbance spectra were obtained between 450 and 4000 cm −1 at a resolution of 4 cm −1 using 20 co-added scans. All spectra presented were baseline corrected and normalized.
X-ray Diffraction (XRD) X-ray powder diffraction (XRD) patterns were recorded using an XRD-diffractometer (Rigaku-Miniiflex II) with a Cu Kα radiation for crystalline phase identification (λ = 0.15405 nm for CuKα). The sample was scanned from 5 to 60 • C.

Scanning Electron Microscopy (SEM)
The morphology of the prepared microparticles was examined using a scanning electron microscope (SEM), type Jeol (JMS-840). All the studied surfaces were coated with carbon black to avoid charging under the electron beam. The instrument was operated at accelerating voltage 20 kV, probe current 45 nA and counting time 60 s.

Differential Scanning Calorimetry (DSC)
A Perkin-Elmer, Pyris 1 differential scanning calorimeter (DSC), calibrated with indium and zinc standards, was employed. A sample of about 10 mg was used for each test, placed in a scaled aluminum pan and heated to 300 • C at a heating rate of 20 • C/min. The sample was held at that temperature for 5 min in order to erase any thermal history. After that it was quenched to 30 • C with liquid nitrogen and scanned immediately to 300 • C at a heating rate of 20 • C/min.

Determination of Amounts of Residual DSU in PLLA Microparticles
In order to determine the amounts of DSU remaining in the PLLA polymer material, microspheres were weighed (~50 mg) and placed in open glass vials at room temperature (25 ± 2 • C) for a period of 4 weeks. Samples at different time intervals such as 0, 1, 2, 3 and 4 weeks were extracted with solvent extraction. 10 mL of methanol were added in each sample and the vials were stoppered. The samples were vortexed for 30 min and then were put in shaking machine for extraction overnight. After the extraction the samples were centrifugated at 4500 rpm for 10 min in order to recover the methanol supernatant containing the released DSU. Then, 1 mL of the organic layer was filtrated using polytetrafluoroethylene (PTFE) 0.22 µm filter and transferred in an autosampler vial. Finally, an aliquot of 1 µL of each extract was subjected to GC-MS analysis. All measurements were performed in triplicate. Quantification of DSU amount on the PLLA microspheres was performed by external calibration (standard solutions at concentrations of 0.01, 0.1, 1.0, 2.5, 5.0 and 10 mg/L in MeOH). Calibration curves were calculated by linear least-squares regression using peak areas (R 2 = 0.99).

Determination of DSU Amount Released from PLLA Microspheres
Determination of the DSU amount released from PLLA microspheres was performed in headspace environment using the Solid Phase Microextraction (SPME) technique. Samples at different time intervals such as 0, 1, 2, 3 and 4 weeks were placed in 20 mL headspace glass vials and sealed immediately with a septum-type cap. Afterwards, the samples were placed in a water bath and left to equilibrate for 10 min. Then, a fused silica SPME fiber coated with polydimethylsiloxane (PDMS) of 100 µm diameter and 1 cm length (SUPELCO, Sigma-Aldrich, Madrid, Spain) was exposed in the headspace environment above the sample and the vials were heated for 45 min at 45 • C. Afterwards, the SPME-fiber was carefully retracted and then inserted directly into the injector of the GC-MS system for 10 min to allow for desorption of the target analyte from the fiber coating. Before measurements, the fiber was conditioned in the injector at 280 • C for 1 h. All samples were analyzed in triplicate. Quantification of DSU was performed by external calibration using standards solutions of DSU. The HS-SPME method used was considered efficient and appropriate, with high recoveries (~100%) and sensitivity (LOQ < 0.005 µg/L) for the DSU. The inter-day and intraday precision expressed, as relative standard deviation (RSD) were lower than 12%, in all cases. Compared to other extraction techniques, SPME technique proved advantageous and environmentally-friendly since it was fast, economic, does not require the use of solvents (volatile compounds are analyzed on the surface of the sample) and thus meet the requirements of "green chemistry".

GC-MS
Gas chromatography (Agilent 6890) equipped with MSD 5973 mass spectrometer (Palo Alto, CA, USA) was used to analyze the extracted pheromone. The capillary column was a nonpolar dimethylpolysiloxane phase (DB-5MS (30 m × 0.25 mm × 0.25 µm film thickness). The flow rate of helium was 1 mL/min in a spitless mode. The run time of the method was 14.5 min. The oven temperature was set initially at 90 • C for 1 min, then ramped to 260 • C at a rate of 20 • C/min. The temperature of the injector was set at 250 • C while the temperature of the MS Quad and MS Source was programmed at 150 • C and at 290 • C, respectively. Confirmation of the DSU was established by the retention time and the presence of the target ions by using the single-ion monitoring (SIM) mode. The characteristic ions selected for the DSU were as follows: m/z 101, m/z 100 and m/z 98.

Synthesis and Characterization of Dacus Pheromone
Concerning 1,7-dioxaspiro [5.5] undecane, as was mentioned previously, was first isolated in female Dacus by Baker et al. [7] while its low quantity for commercial use lead the researchers to synthesize it in the lab. First, in 1983 it was synthesized by two independent groups [26,27]. Numerous studies have been reported in the literature thereafter concerning the synthesis of pheromone including asymmetric synthesis [28]. Kranidiotis et al. [24] proposed a novel short synthesis of racemic 1,7-dioxaspiro [5.5]undecane, named (±)-olean (Figure 1), through cross metathesis resulting in a cheap and easy to follow procedure. In the proper study, a new, simple and efficient synthesis of 1,7-dioxaspiro [5.5]undecane in five steps was developed starting from butane-1,4-diol. Although many synthetic approaches towards olean syntheses have been reported in literature, including their asymmetric syntheses [28], we decided to developed a new simple and efficient synthesis of olean in five steps, starting from butane-1,4-diol, as outlined in Scheme 1. Firstly, butane-1,4-diol was monobenzylated using benzyl bromide as limiting reagent in 99% yield (based on benzyl bromide). The primary hydroxyl group was then replaced by a bromine atom by a standard procedure to give bromide 2 in 80% yield and addition of the respective Grignard reagent to ethyl formate afforded good yields of alcohol 3. Subsequent oxidation of 3 with pyridinium chlorocromate (PCC) yielded quantitatively the respective ketone, which upon debenzylation with catalytic hydrogenation led to the spontaneous cyclization of the intermediately formed dihydroxyketone, to give the desired racemic olean in 80% yield. The overall yield of converting compound 1 to olean was 37%.
All compounds prepared were of high purity and characterized by their spectral and analytical data. Final (±)-olean as well as intermediate products gave accurate and clear 1 H and 13 C NMR spectra without the presence of any impurity.

Characterization of Prepared Microparticles
Microparticles were prepared according to o/w technique as described previously [16,18,19]. SEM ( Figure 2) was used in order to verify microparticles formation as well as their surface morphology. As can be seen, microparticles were successfully synthesized with sizes ranged between 1 and 2.5 μm, while no agglomeration was observed. Small differences of about 0.3 μm was observed concerning the DSU content with their sizes increased as quantity of DSU increased. Surface morphology showed to be smooth, owing to the polymer used, while no porous were observed. Although many synthetic approaches towards olean syntheses have been reported in literature, including their asymmetric syntheses [28], we decided to developed a new simple and efficient synthesis of olean in five steps, starting from butane-1,4-diol, as outlined in Scheme 1. Although many synthetic approaches towards olean syntheses have been reported in literature, including their asymmetric syntheses [28], we decided to developed a new simple and efficient synthesis of olean in five steps, starting from butane-1,4-diol, as outlined in Scheme 1. Firstly, butane-1,4-diol was monobenzylated using benzyl bromide as limiting reagent in 99% yield (based on benzyl bromide). The primary hydroxyl group was then replaced by a bromine atom by a standard procedure to give bromide 2 in 80% yield and addition of the respective Grignard reagent to ethyl formate afforded good yields of alcohol 3. Subsequent oxidation of 3 with pyridinium chlorocromate (PCC) yielded quantitatively the respective ketone, which upon debenzylation with catalytic hydrogenation led to the spontaneous cyclization of the intermediately formed dihydroxyketone, to give the desired racemic olean in 80% yield. The overall yield of converting compound 1 to olean was 37%.
All compounds prepared were of high purity and characterized by their spectral and analytical data. Final (±)-olean as well as intermediate products gave accurate and clear 1 H and 13 C NMR spectra without the presence of any impurity.

Characterization of Prepared Microparticles
Microparticles were prepared according to o/w technique as described previously [16,18,19]. SEM (Figure 2) was used in order to verify microparticles formation as well as their surface morphology. As can be seen, microparticles were successfully synthesized with sizes ranged between 1 and 2.5 μm, while no agglomeration was observed. Small differences of about 0.3 μm was observed concerning the DSU content with their sizes increased as quantity of DSU increased. Surface morphology showed to be smooth, owing to the polymer used, while no porous were observed. Firstly, butane-1,4-diol was monobenzylated using benzyl bromide as limiting reagent in 99% yield (based on benzyl bromide). The primary hydroxyl group was then replaced by a bromine atom by a standard procedure to give bromide 2 in 80% yield and addition of the respective Grignard reagent to ethyl formate afforded good yields of alcohol 3. Subsequent oxidation of 3 with pyridinium chlorocromate (PCC) yielded quantitatively the respective ketone, which upon debenzylation with catalytic hydrogenation led to the spontaneous cyclization of the intermediately formed dihydroxyketone, to give the desired racemic olean in 80% yield. The overall yield of converting compound 1 to olean was 37%.
All compounds prepared were of high purity and characterized by their spectral and analytical data. Final (±)-olean as well as intermediate products gave accurate and clear 1 H and 13 C NMR spectra without the presence of any impurity.

Characterization of Prepared Microparticles
Microparticles were prepared according to o/w technique as described previously [16,18,19]. SEM (Figure 2) was used in order to verify microparticles formation as well as their surface morphology. As can be seen, microparticles were successfully synthesized with sizes ranged between 1 and 2.5 µm, while no agglomeration was observed. Small differences of about 0.3 µm was observed concerning the DSU content with their sizes increased as quantity of DSU increased. Surface morphology showed to be smooth, owing to the polymer used, while no porous were observed.
FT-IR was further used to verify possible bond formation between PLLA and DSU. As shown in Figure 3, PLLA showed a single peak at 1760 cm −1 owing to carbonylic bond -C=O [18] and DSU showed a double peak at 2938 and 2869 cm −1 owing to C-H stretching vibrations and one at 991 cm −1 due to C-O-C vibrations [29]. Microparticles of 5, 10 and 20% DSU did not show significant frequency shifts, while peaks appeared at 990 cm −1 indicating the presence of pheromone in formed microparticles. FT-IR was further used to verify possible bond formation between PLLA and DSU. As shown in Figure 3, PLLA showed a single peak at 1760 cm −1 owing to carbonylic bond -C=O [18] and DSU showed a double peak at 2938 and 2869 cm −1 owing to C-H stretching vibrations and one at 991 cm −1 due to C-O-C vibrations [29]. Microparticles of 5, 10 and 20% DSU did not show significant frequency shifts, while peaks appeared at 990 cm −1 indicating the presence of pheromone in formed microparticles. XRD was used in order to determine the crystallinity of PLLA microparticles before and after DSU's encapsulation. PLLA is a semicrystalline polymer, as has been previously reported [19] and its recorded pattern is shown in Figure 4. Two characteristic peaks of PLLA at 16.6 and 18.8 deg were present, while after DSU encapsulation there was a reduction to intensity of the peaks. As the amount XRD was used in order to determine the crystallinity of PLLA microparticles before and after DSU's encapsulation. PLLA is a semicrystalline polymer, as has been previously reported [19] and its recorded pattern is shown in Figure 4. Two characteristic peaks of PLLA at 16.6 and 18.8 deg were present, while after DSU encapsulation there was a reduction to intensity of the peaks. As the amount of DSU increased the reduction was much higher and this is an indication that the crystallinity of PLLA was reduced, probably because DSU could act as plasticizer to PLLA. Furthermore, higher the encapsulated amount resulted in enhancement of the proper effect. In order to confirm this, DSC was used as a further study and also to detect thermal properties of prepared microparticles. wavenumbers (cm -1 ) XRD was used in order to determine the crystallinity of PLLA microparticles before and after DSU's encapsulation. PLLA is a semicrystalline polymer, as has been previously reported [19] and its recorded pattern is shown in Figure 4. Two characteristic peaks of PLLA at 16.6 and 18.8 deg were present, while after DSU encapsulation there was a reduction to intensity of the peaks. As the amount of DSU increased the reduction was much higher and this is an indication that the crystallinity of PLLA was reduced, probably because DSU could act as plasticizer to PLLA. Furthermore, higher the encapsulated amount resulted in enhancement of the proper effect. In order to confirm this, DSC was used as a further study and also to detect thermal properties of prepared microparticles.   As was already reported, PLLA is a semicrystalline polymer and exhibited a glass transition (T g ) and melting temperature (T m ) at 69.9 • C and at 154.2 • C, respectively, while cold crystallization (T cc ) was also observed at 127.9 • C ( Figure 5). These are in good agreement with the corresponding values reported in literature [18,25]. Slight changes were observed in DSC thermographs of prepared microparticles after DSU incorporation. In brief, T g values were reduced with the increase of DSU from 69.9 of neat PLLA to 61.8, 61.1 and 60.8 • C, of 5, 10 and 20% w/w, respectively. This is an indication that DSU due to its low molecular weight could act as plasticizer for PLLA polymer, which is in good agreement with XRD results. Reduction in characteristic T cc and T m values of PLLA was also observed in prepared microparticles. In brief, T m values of PLLA showed reduction from 154.2 • C to 151.3, 150.6 and 151.0 • C for microparticles containing 5, 10 and 20 wt% DSU, respectively, without showing any specific trend. Concerning T cc values reduction was observed from 127.9 • C of PLLA to 124.6, 122.0 and 123.1 • C, respectively. Reduction in T cc value of PLLA indicates that DSU facilitates cold crystallization procedure, mainly due to looser chain formation of polymeric entanglements.
Thermal degradation of each formulation was further evaluated with thermogravimetric analysis (TGA). As shown in Figure 6, PLLA's thermal decomposition starts at 288 • C with the first stage ending at 310 • C showing a mass loss of about 1.5%, followed by a second stage which ended at 404 • C while no further thermal decomposition was observed. Thermal decomposition of PLLA microparticles containing DSU was slightly different. PLLA microparticles containing 5% DSU started to decompose at 226 • C with a mass loss of about 4%, probably attributed to the pheromone mass loss, due to the fact that its boiling point is 194 • C. The first degradation stage lasted at 263 • C, while followed by a second stage until 351 • C. From that point after there was no significant mass loss and the mass residue was approximately 5%. For microparticles of PLLA containing 10% DSU decomposition started at 190 • C and lasted at 210 • C, showing mass loss of about 8%, and a second stage from 210 • C till 359 • C with remaining mass of about 5%. Analogous were the results for PLLA microparticles containing 20% DSU; an initial step till 203 • C, with a mass loss of 15%, and a second one till 364 • C and remaining mass 5.5%. From all these thermograms it is clear that by increasing the amount of DSU the maximum decomposition temperature of PLLA progressively shifted to lower temperatures due to the high volatility of DSU. TGA thermographs constitute an initial estimation concerning DSU concentration in microparticles. Hence, due to the fact that DSU evaporated easily and TGA did not show high sensitivity, GC-MS analysis was further used. and melting temperature (Tm) at 69.9 °C and at 154.2 °C, respectively, while cold crystallization (Tcc) was also observed at 127.9 °C ( Figure 5). These are in good agreement with the corresponding values reported in literature [18,25]. Slight changes were observed in DSC thermographs of prepared microparticles after DSU incorporation. In brief, Tg values were reduced with the increase of DSU from 69.9 of neat PLLA to 61.8, 61.1 and 60.8 °C, of 5, 10 and 20% w/w, respectively. This is an indication that DSU due to its low molecular weight could act as plasticizer for PLLA polymer, which is in good agreement with XRD results. Reduction in characteristic Tcc and Tm values of PLLA was also observed in prepared microparticles. In brief, Tm values of PLLA showed reduction from 154.2 °C to 151.3, 150.6 and 151.0 °C for microparticles containing 5, 10 and 20 wt% DSU, respectively, without showing any specific trend. Concerning Tcc values reduction was observed from 127.9 °C of PLLA to 124.6, 122.0 and 123.1 °C, respectively. Reduction in Tcc value of PLLA indicates that DSU facilitates cold crystallization procedure, mainly due to looser chain formation of polymeric entanglements. Thermal degradation of each formulation was further evaluated with thermogravimetric analysis (TGA). As shown in Figure 6, PLLA's thermal decomposition starts at 288 °C with the first stage ending at 310 °C showing a mass loss of about 1.5%, followed by a second stage which ended at 404 °C while no further thermal decomposition was observed. Thermal decomposition of PLLA microparticles containing DSU was slightly different. PLLA microparticles containing 5% DSU started to decompose at 226 °C with a mass loss of about 4%, probably attributed to the pheromone mass loss, due to the fact that its boiling point is 194 °C. The first degradation stage lasted at 263 °C, while followed by a second stage until 351 °C. From that point after there was no significant mass loss and the mass residue was approximately 5%. For microparticles of PLLA containing 10% DSU decomposition started at 190 °C and lasted at 210 °C, showing mass loss of about 8%, and a second stage from 210 °C till 359 °C with remaining mass of about 5%. Analogous were the results for PLLA microparticles containing 20% DSU; an initial step till 203 °C, with a mass loss of 15%, and a second one till 364 °C and remaining mass 5.5%. From all these thermograms it is clear that by increasing the

DSU Release from PLLA Microparticles
GC-MS analysis was conducted as referred in Section 2.4.2. Table 1 shows microparticles yield (%), pheromone loading (%) and encapsulation efficiency (%) of microparticles prepared. The proper values are referring to the zero day and the analysis conducted immediately after microparticles

DSU Release from PLLA Microparticles
GC-MS analysis was conducted as referred in Section 2.4.2. Table 1 shows microparticles yield (%), pheromone loading (%) and encapsulation efficiency (%) of microparticles prepared. The proper values are referring to the zero day and the analysis conducted immediately after microparticles formation in order to avoid DSU release during storage. As can be observed, microparticles showed high yield values, over 80% for all three formulations, with that of 10% DSU reaching up to 91.5%, while no specific sequence was observed. Pheromone loading quantification was conducted according to SPME and found that DSU was present in 4.8, 9.1 and 16.8% in microparticles containing 5, 10 and 20% w/w DSU. The proper results were analogous to the ones found by TGA analysis, where DSU was found to be 4, 8 and 15%.  Figure 7 shows the remaining mass of DSU after liquid extraction procedure at 0, 1, 2, 3 and 4 weeks. As can be observed microparticles containing 5% w/w DSU showed a total mass loss in 1 week with a reduction from about 2.5 mg to 0.2 mg without any change thereafter meaning that the quantity of the pheromone remained was the total quantity of DSU was successfully released from microparticles. Concerning concentration 10% w/w DSU it was found that the main reduction in DSU content made in the first week with a loss of about 3.25 mg, while in the second week there was also observed a reduction in DSU content with an additional mass loss of 0.75 mg. Additional losses of about 0.3 and 0.1 mg was observed in the third and fourth respectively with a remaining mass of 0.08 mg. Finally, formulation of 20% w/w DSU showed to half reduce DSU content in the first week, an additional reduce of about 2.5 mg in the second week and about 1 and 0.5 mg in the third and fourth week respectively. It has to be mentioned that in all formulations the remaining mass of DSU was below 0.1 mg. Figure 8 shows the percentage release of DSU form PLLA microparticles conducted by SPME technique. As can be observed microparticles containing 5 and 10% w/w DSU showed a release reached at 90 and 80% in the first week with an increase of about 2 and 10% in the second week, reaching 92 and 90% respectively without any significant changes thereafter. The initial burst release probably arose from the quantity of DSU remaining on the surface of the microparticles, allowing for easier release. The proper results are in accordance with the ones revealed by LE technique where, as was described previously, the total quantity of DSU was actually released in the first week for microparticles containing 5% and in the second week, with a slight increase between the two first weeks, for microparticles containing 10% DSU. Microparticles containing 20% w/w DSU showed a different profile. In brief, a sustained release profile was observed with DSU release reaching 55% in the first week, 83% in the second week, 94% in the third week and 99% in the fourth week. Concerning the proper release, it is believed that the initial release of 55% observed in the first week in probably owing to DSU release remained to the surface of microparticles, while from that time after the release could be attributed to pores formed in the surface and channels formed to the inner of microparticles renders the release easier. Finally, the recorded results are also in agreement with that obtained by LE procedure which also showed a gradual reduction in DSU mass. From these it is clear that microparticles containing 20 wt% DSU could be the ideal carrier to control Dacus oleae population for about 4 weeks. content made in the first week with a loss of about 3.25 mg, while in the second week there was also observed a reduction in DSU content with an additional mass loss of 0.75 mg. Additional losses of about 0.3 and 0.1 mg was observed in the third and fourth respectively with a remaining mass of 0.08 mg. Finally, formulation of 20% w/w DSU showed to half reduce DSU content in the first week, an additional reduce of about 2.5 mg in the second week and about 1 and 0.5 mg in the third and fourth week respectively. It has to be mentioned that in all formulations the remaining mass of DSU was below 0.1 mg.  Figure 8 shows the percentage release of DSU form PLLA microparticles conducted by SPME technique. As can be observed microparticles containing 5 and 10% w/w DSU showed a release reached at 90 and 80% in the first week with an increase of about 2 and 10% in the second week, reaching 92 and 90% respectively without any significant changes thereafter. The initial burst release probably arose from the quantity of DSU remaining on the surface of the microparticles, allowing for easier release. The proper results are in accordance with the ones revealed by LE technique where, as was described previously, the total quantity of DSU was actually released in the first week for microparticles containing 5% and in the second week, with a slight increase between the two first weeks, for microparticles containing 10% DSU. Microparticles containing 20% w/w DSU showed a different profile. In brief, a sustained release profile was observed with DSU release reaching 55% in the first week, 83% in the second week, 94% in the third week and 99% in the fourth week. Concerning the proper release, it is believed that the initial release of 55% observed in the first week in probably owing to DSU release remained to the surface of microparticles, while from that time after the release could be attributed to pores formed in the surface and channels formed to the inner of microparticles renders the release easier. Finally, the recorded results are also in agreement with that obtained by LE procedure which also showed a gradual reduction in DSU mass. From these it is clear that microparticles containing 20 wt% DSU could be the ideal carrier to control Dacus oleae population for about 4 weeks.

Conclusions
In this study, the sexual pheromone of the insect Bactrocera oleae (DSU) was successfully synthesized following a novel, facile, five step method. The synthesized DSU was characterized by 1 H and 13 C NMR and with HPMS (ESI) showing its successful synthesis. DSU was further used in PLLA microparticles' preparation at 5, 10 and 20 wt%. As was found by FT-IR and DSC measurements, DSU was successfully encapsulated to microparticles. Even though some interactions are not taking place between DSU and PLLA reactive groups, it was found that DSU due to its low molecular weight could act as plasticizer to PLLA matrix. GC-MS was used for quantification of remaining DSU in microparticles at weeks 0, 1, 2, 3 and 4 and release profile was studied. Results showed that for microparticles containing 5 and 10% DSU release practically lasted in 1 and 2 weeks respectively, while for microparticles with 20% DSU release showed a controlled profile lasted in 4

Conclusions
In this study, the sexual pheromone of the insect Bactrocera oleae (DSU) was successfully synthesized following a novel, facile, five step method. The synthesized DSU was characterized by 1 H and 13 C NMR and with HPMS (ESI) showing its successful synthesis. DSU was further used in PLLA microparticles' preparation at 5, 10 and 20 wt%. As was found by FT-IR and DSC measurements, DSU was successfully encapsulated to microparticles. Even though some interactions are not taking place between DSU and PLLA reactive groups, it was found that DSU due to its low molecular weight could act as plasticizer to PLLA matrix. GC-MS was used for quantification of remaining DSU in microparticles at weeks 0, 1, 2, 3 and 4 and release profile was studied. Results showed that for microparticles containing 5 and 10% DSU release practically lasted in 1 and 2 weeks respectively, while for microparticles with 20% DSU release showed a controlled profile lasted in 4 weeks. The results are promising for using the proper microparticles as innovative formulations in Dacus oleae population control.