Use of X-ray irradiation for inactivation of Aspergillus in cannabis flower

Strain preparation

The Aspergillus strains used in this study (Table 1) were grown for 2 to 5 days at 30°C on potato dextrose agar (PDA). Spores were harvested from PDA plates by washing with 10 mL sterile 0.05% Tween 20 in water and quantified by hemocytometer cell counting. Spore suspensions were then normalized and serially diluted to the desired concentrations.

Aspergillus enrichment and detection by real-time PCR

After X-ray treatments, potato dextrose broth containing 0.05% chloramphenicol was added to each cannabis sample to make a 1:25 dilution (1 g sample in 24 mL media). Samples were then incubated at 30°C for 48 ± 4 hours. After incubation, 5 mL of sample enrichment was removed for PCR analysis.

The 5 mL sample enrichments were centrifuged at 5000 rpm for 2 minutes and the supernatant was discarded. Pellets were resuspended in 500 μL lysis buffer [41] (400 mM Tris-HCl [pH 8.0], 60 mM EDTA [pH 8.0], 150 mM NaCl, 1% sodium dodecyl sulfate) and added to a screw-cap microcentrifuge tube with sterile glass beads (Sigma G1277, 212–300 μm) filled to approximately the 0.1 mL line.

Bead-beating was performed at 6m/s for 1 minute on a FastPrep24-5G (M.P. Biomedicals, Santa Ana, CA), after which samples were placed on ice for 1 minute. DNA extraction continued as described by Liu et al. [41] from step (ii) with minor modifications. DNA pellets were resuspended in 50 μL sterile distilled water, and 2 μL was used for real-time PCR.

PCR reactions were performed using a QuantStudio 5 (Applied Biosystems, Foster City, CA) in a 20 μL reaction volume containing TaqPath ProAmp Multiplex Master Mix (Applied Biosystems Cat# A30868), 1 μL Thermo Fisher Aspergillus multiplex v2 (Custom TaqMan Aspergillus Kit v2, Cat# A43213C), and 2 μL DNA. The following cycling conditions were used: 95°C for 5 minutes, followed by 40 cycles of 95°C for 5 seconds and 63°C for 30 seconds. Reporter dyes were used with the following targets: FAM (fumigatus), VIC (flavus), ABY (terreus), and JUN (niger). Mustang Purple was used as a passive reference dye.

Real-time PCR results were analyzed using QuantStudio Design and Analysis Software v1.5.1. Thresholds for each target were set as follows: niger (0.2), fumigatus (0.2), flavus (0.8), terreus (0.8).

Viability of Aspergillus in the cannabis sample enrichments was determined by plating onto PDA using a 10 μL loop and incubating for up to 5 days at 30°C. Plates were examined for typical Aspergillus growth for the appropriate species.

X-ray irradiation and Aspergillus viability

To determine the dosage required to inactivate A. niger, A. fumigatus, A. flavus, and A. terreus spores, large amounts of spores (>10⁶), from each Aspergillus species, were spiked into 1 gram of dried cannabis flower in Whirlpak bags. The spiked cannabis samples were then exposed to 2.0, 2.5, or 5.0 kGy of X-ray irradiation. Following irradiation, all samples were tested and viability confirmed as described above.

In a second assay, 1 gram cannabis flower samples were inoculated with low (10² spores), medium (10³ spores), or high (10⁴ spores) amounts of A. niger, A. fumigatus, A. flavus, or A. terreus spores. “Treated” samples were exposed to 2.5 kGy of X-ray irradiation. Similarly, inoculated control samples were prepared and received no x-ray exposure and served as “untreated” samples. All samples were tested in triplicate.

In a third assay, for a larger scale experiment, two 100 g cannabis flower samples were spiked with 10⁶ A. niger spores/100 g flower. One sample was then exposed to 2.5 kGy of X-ray irradiation and the other left untreated. Two 10 g subsamples were randomly taken from each sample (including an additional 100 g matrix control) and tested as described above.

Sample preparation for chemical analysis

Dried cannabis flowers (trimmed buds) were ground and homogenized using GenoGrinder from SPEX SamplePrep (Metuchen, NJ), and seven bags each containing 3 grams of ground flowers were prepared for X-ray irradiation treatment. Ground cannabis flower samples were treated at six different X-ray irradiation dosage level (0.5, 1.0, 1.5, 2.0, 2.5 and 5.0 kGy). A triplicate of 200 mg samples was weighed out from each X-ray treated samples as well as the untreated sample. The samples were extracted with 40 mL extraction solvents (80 acetonitrile: 20methanol, v/v), sonicated for 30 min, followed by centrifugation at 3900 rpm for 15 min. The supernatant was filtered through a 0.25 μm PTFE filter and further diluted 200-fold and 400-fold, respectively before loading onto the instrument for qualitative and quantitative analyses. A seven-point calibration curve from 20 ppb to 2000 ppb was used to determine the concentration of the cannabinoids in the samples. Isotopically labeled THC-d₃ was added to each calibration standard and all samples to serve as internal standard. Quality control samples were included in the batch to ensure accuracy and precision of the method.

Cannabinoid quantitative analysis by UHPLC-MS/MS

The quantitative analysis of eight different cannabinoids (namely, CBDA, CBD, THCA, delta9-THC, CBN, CBG, THCV and CBC) were performed on a SCIEX Exion UHPLC system coupled with a triple quadrupole mass spectrometer (4500) with an ESI source (Framingham, MA). SCIEX Analyst software (1.7.0) was used to control the instrument and collect data. All eight cannabinoids reference standards CBDA, CBD, THCA, delta9-THC, CBN, CBG, THCV and CBC and the internal standards (THC-d3) were purchased from Cerilliant (Round Rock, TX). LCMS grade Methanol, acetonitrile, water and formic acid were purchased from Fisher Scientific.

The LC column used for this method was a Cortecs UPLC C18 column (100mm× 2.1mm I.D., 1.6 μm) from Waters (Milford, MA). The column oven temperature was set at 35°C. The mobile phases consisted of (A) 0.05% formic acid in water and (B) 0.05% formic acid in acetonitrile. The following gradient was used to achieve chromatographic separation of the cannabinoids at a flow rate of 0.25 ml/min: 0–8min, 70 to 80% B; 8–10 min, 80 to 100% B, followed by a 4-min washing procedure with 100% B and a re-equilibration period of 4 min with initial conditions. The total run time was 18 min for each sample. The injection volume was 2 μL. The autosampler was maintained at 15°C. For the MS/MS parameters, both positive and negative mode were used for detecting different cannabinoids: CBD, delta9-THC, CBN, CBG, THCV and CBC were detected using positive mode and the acidic cannabinoids CBDA and THCA were detected using negative mode. Ion spray voltage was set to 4500 for the positive mode and -4500 for the negative mode. Curtain gas was set to 40 psi. Source Temperature (TEM) was 500°C. Ion source gas 1 and 2 (GS1 and GS2) were both set at 50 psi. Two different ion transitions were used for each cannabinoid.

X-ray irradiation with quantitative spike levels

No viability was observed for any of the Aspergillus spp. in the samples exposed to 2.5 kGy, regardless of inoculation level. Without X-ray irradiation, Aspergillus growth was observed even at the lowest spike levels. At medium and high spike levels, DNA from Aspergillus spores were detectable by PCR, even after X-ray exposure. In samples without X-ray exposure irradiation, respective Aspergillus spp. were detected by PCR regardless of spike level, see Tables ​Tables33–6. Irradiated medium and high spike samples resulted in detectable Ct values although with later cycle thresholds than comparable untreated samples. A sample was considered “positive”, DNA detected, for an Aspergillus target if fluorescent curves crossed the cycle threshold (Ct) line ≤40. A Ct of zero means that the fluorescent curve did not cross the cycle threshold.

Similar results were observed in the 100 g scale-up experiment: each 10 g subsample exposed to 2.5 kGy of X-rays showed no A. niger viability, while those without X-ray exposure had Aspergillus growth, See Table 7.

Cannabinoids profile by LC-MSMS

A total of twenty-one samples were used in this study—three untreated cannabis flower samples and three replicate samples from each of the six X-ray dosage levels, respectively.

Table 8 shows the average of the cannabinoid concentrations of the three replicate samples before and after the X-ray irradiation treatment. The top two most abundant cannabinoids in the tested flower samples were THCA and delta9-THC, respectively. The slight differences in concentration of THCA/delta9-THC at different levels are mainly due to the natural inhomogeneity of the cannabis flower sample and the measurement uncertainty for all analytical methods. A trend test across different treatment groups was performed on STATA version 17.0 (StataCorp) for potential cannabinoids profile changes after X-ray irradiation. We set the level of significance as p < 0.05. No significant trends were observed for THCA and delta9-THC concentrations.

Concentrations for CBDA, THCV, CBG and CBC are less than the reporting limit (1.6mg/g or 0.16%) but mostly unchanged for each X-ray dosage level. There was no CBD identified in the tested cannabis flower samples.

The temperature in the X-ray chamber was monitored during the X-ray irradiation process, which was slightly elevated to around 28°C compared to the 23°C at the beginning. This slight elevation of temperature did not seem to cause accelerated decarboxylation of the THCA to THC nor degradation of the THC to CBN in the sample, as there is no trend observed for changes in the THCA and THC concentrations. Fig 1 shows the average THCA and delta9-THC concentrations of the flower samples treated at different dosage levels, with error bars calculated using standard deviation of the three replicates for each level. It is reasonable to conclude that the X-ray irradiation has minimal impact on the THCA and delta9-THC of the cannabis flower samples.

Qualitative cannabinoids profile by GC-MS

To confirm the findings of cannabinoids profile by LC-MSMS, GC-MS screen method was also used in this study. Four cannabis flower samples ‒ one untreated and three treated with 1.0, 2.5 and 5.0 kGy dose levels were analyzed to determine if cannabinoid and terpene profiles had changed after X-ray irradiation. A second set of samples were used to confirm the findings. The peak area percentages of the compounds generated from GC-MS analysis were used for the qualitative analysis. Peak area percentage of each peak roughly represents the composition and amount of analyte (e.g., Delta9-THC) observed in the sample.

The major cannabinoids found in flower samples were Delta9-THC (~70% peak area), CBG (~ 3% peak area), CBC (2.5% peak area), CBN (2.5% peak area), THCV (0.7% peak area), and cannabifuran (0.3% peak area) (Fig 2). Due to high temperature on heated GC-MS injection port, THCA, CBDA and other acid form of cannabinoids were not observed by GC-MS as they were mostly decarboxylated to the neutral cannabinoids such as THC and CBD. We did not observe any changes for Delta9-THC, CBG, CBC, and THCV. There was a slight increase in CBN amount as the treatment doses increased. CBN is an oxidation and degradation byproduct of the Delta9-THC and the slight increase may be due to slight increase in temperatures at higher levels of the X-ray treatment. There was also a slight increase in cannabifuran amount at the highest treatment dose level (5.0 kGy). The qualitative results observed were not tested for statistical significance. The cannabinoid profile by GC-MS screen method is consistent with the results found using LC-MSMS quantitative analysis.

We would like to thank Rad Source Technologies staff for providing us with the X-ray equipment used to conduct this study.