30 September 2025, Volume 45 Issue 9
    

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    Ingredient Analysis
  • Establishment of an indirect competitive ELISA immunosorbent assay for determination of cinobufagin in abdominal pain water*
    SUN Ying, ZHANG Xiu-bo, LIU Cheng-linzi, XIANG Qian, XIE Wei, WANG Jing, HU Chang-yuan, GAO Meng-ge, DUAN He-bo, LI Hua-yuan
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1465-1473. https://doi.org/10.16155/j.0254-1793.2025-0145
    Abstract ( ) Download PDF ( )   Knowledge map   Save
    Objective: To prepare monoclonal antibody (McAb) that can specifically recognize cinobufagin (CBG), establish a specific and rapid quantitative detection method for CBG, and apply it to quantitative detection of CBG in abdominal pain water. Methods: :BALB/c mice were immunized by artificial antigen, which was prepared by CBG coupling with carrier protein, and McAb for CBG was prepared through hybridoma technique. An indirect competitive enzyme-linked immunosorbent assay (icELISA) based on McAb for CBG was developed, and used for CBG quantification in abdominal pain water. Results: Two hybridoma cell lines (C1 and C6) were selected, with the titer of 1 ∶ 90 000 and 1 ∶ 810 000, respectively. icELISA based on C6 was established, with sensitivity (IC50) of 15.92 ng · mL-1, detection range (IC20-IC80) of 2.45-103.42 ng · mL-1, and detection limit (IC10) of 1.32 ng · mL-1.The cross-reactivity of this assay with resibufogenin and bufalin were 9.37% and 0.03%, respectively, negligible cross-reactivity were found in deoxycholic acid and androsterone. The intra-assay and inter-assay recovery rates of CBG spiked in samples were 92%-115% and 92%-106%, respectively, the precision test showed that the intra-assay and inter-assay RSD of detected CBG concentration were less than 10%. The contents of CBG in 5 batches of abdominal pain water were detected by the established icELISA, ranging from 5.06-6.07 μg · mL-1, which were consistent with detection results of HPLC. Conclusion: In this study, McAb specific to CBG was prepared, a specific and sensitive icELISA was developed. The quantification of CBG in 5 batches of abdominal pain water using this method showed good inter-batch consistency.
  • Determination of related substances in abemaciclib active pharmaceutical ingredient by HPLC*
    LIU Yun, YANG Ben-xia, FAN Li-jia
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1474-1482. https://doi.org/10.16155/j.0254-1793.2025-0351
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    Objective: To establish an HPLC method for determination of related substances in abemaciclib. Methods: :The gradient elution was carried out through an InfinityLab Poroshell 120 EC-C18 column (150 mm×4.6 mm,4 μm) with tetrabutylammonium hydroxide aqueous solution (adjusted to pH 10.0 with formic acid) as the mobile phase A and acetonitrile as the mobile phase B at a flow rate of 1.2 mL · min-1. The detection wavelength was set at 296 nm, and the column temperature was 30 ℃. The injection volume was 10 μL. Results: Abemaciclib can be completely separated from all impurities (separation degree≥2.45). The test solution was stable for at least 7 d. The limits of quantitation of impurities Ⅰ-Ⅶ were all 0.04%. The 7 impurities showed good linearity (r≥0.997 6)in the tested ranges. The average recovery rates of the impurities were in the range of 94.7%-101.7%, with the RSD≤2.2%. The method showed high precision and stability. Conclusion: The method, with high sensitivity, specificity, and accuracy, can be used for the determination of the related substances in abemaciclib.
  • Quality evaluation of Erchen pills by HPLC fingerprint combined with chemometrics and multi-component quantitative determination*
    LIU Ying-xin, LIU Li-li, CHEN Rong, YANG Hui, LU Xin-tian, MAO Qun-fang, QIU Yan-ming
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1483-1495. https://doi.org/10.16155/j.0254-1793.2025-0261
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    Objective: To establish the HPLC fingerprint and the multi-component quantitative determination method for Erchen pills and evaluate the quality of multiple batches of formulations from different manufacturers through chemometric methods. Methods: :HPLC fingerprints of Erchen pills were established and subjected to similarity evaluation. The separation was performed on an Agilent ZORBAX Eclipse Plus C18 column (250 mm×4.6 mm, 5 μm) with a mobile phase of acetonitrile and 0.1% phosphoric acid aqueous solution under a gradient elution program. The detection wavelength, column temperature, and flow rate were set at 270 nm, 25 ℃, and 1.0 mL · min-1,respectively. Hierarchical clustering analysis (HCA) and principal component analysis (PCA) were performed to analyze the quality of the formulations from different manufacturers. The content of six active ingredients—narirutin, hesperidin, isosakuranetin 7-O-rutinoside, glycyrrhizic acid, nobiletin, and licoisoflavone B in different batches of Erchen pills was determined by HPLC. The quality was evaluated by grey correlation analysis (GCA). Results: HPLC fingerprints were established for 18 batches of Erchen pills, and a total of 15 common peaks were calibrated, with six common chromatographic peaks identified. HCA and PCA demonstrated significant quality disparities among samples from different manufacturers. The content of narirutin, hesperidin, isosakuranetin 7-O-rutinoside, glycyrrhizic acid, nobiletin, and licoisoflavone B in 18 batches of Erchen pills samples ranged from 0.997 5 to 2.781 3 mg · g-1,0.825 2 to 4.794 1 mg · g-1, 0.110 1 to 0.384 5 mg · g-1, 0.551 5 to 2.718 1 mg · g-1, 0.016 8 to 0.428 4 mg · g-1, and 0.010 5 to 0.100 1 mg · g-1, respectively. The results of GCA and PCA were basically consistent in the overall trend. Conclusion: The established HPLC fingerprint and multi-component content determination method are accurate and reliable, and they can be combined with chemometric methods for the quality evaluation of Erchen pills.
  • Determination of 14 elemental impurities in azlocillin sodium for injection by ICP-MS
    WU Jing-ping, YANG Zhi-qiang, ZHENG Ting
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1496-1503. https://doi.org/10.16155/j.0254-1793.2025-0258
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    Objective: To develop an inductively coupled plasma-mass spectrometry (ICP-MS) method for 14 elemental impurities (Cd, Pb, As, Hg, Co, V, Ni, Sb, Ba, Cu, Cr, Fe, Zn, and Mn) in azlocillin sodium for injection and evaluate the influences of Cu, Zn, and Hg (elements prohibited for combination) on the stability of azlocillin. Methods: :Samples were digested by microwave. ICP-MS was employed for full quantitative analysis, with the power of 1 550 W, a carrier gas flow rate of 0.8 L · min-1, an atomization gas flow rate of 1.11 L · min-1, a cooling gas flow rate of 14 L · min-1, 5 times of signal measurement, and sampling depth of 8 mm. The internal standard solution of Bi, Ge, In, and Sc were used for matrix effect correction via the standard curve method. Results: The 14 elements showed good linearities, with the correlation coefficients (r) being all above 0.997. The detection limits of elements were in the range of 0.001-0.131 μg · g-1. The average recoveries of the elements were in the range of 92.4%-112.8%. The RSDs of the precision test were in the range of 1.3%-4.2% and those of the repeatability test were in the range of 1.8%-6.0%, all of which met the requirements of methodological validation. In 24 batches of samples, the content of 14 elements was all in the acceptable ranges. The compatibility study results indicated that the element levels were all less than permitted daily exposure. Among the elements prohibited for combination, Zn had higher relative content, which was also below the exposure limit and had no correlation with the content of azlocillin. Conclusion: The elemental impurities in sodium aloxicillin for injection are well controlled, and the risk of catalytic degradation of aloxicillin due to elements prohibited for combination is small. The proposed method is accurate and sensitive, providing a reference for the risk assessment of elemental impurities in other similar drugs.
  • Determination of potassium sorbate content in pharmaceutical excipients using indirect 1H qNMR method
    CHEN Xin-qi, WEN Jing, ZHANG Jia-yi, ZHANG Mei, JIAO Xiao-lin, WANG Wei
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1504-1510. https://doi.org/10.16155/j.0254-1793.2025-0256
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    Objective: To establish a quantitative nuclear magnetic resonance hydrogen spectroscopy (1H qNMR) method for indirectly determining the content of potassium sorbate, in order to apply it to the determination of the content of other similar pharmaceutical excipients and compounds. Method: DMSO was used as a reference substance and dissolved in heavy water to form a reference solution. An appropriate amount of the test substance (potassium sorbate) and the standard substance (maleic acid) were mixed with equal volumes of the reference solution to prepare samples, and the 1H qNMR were measured respectively. Based on the integration of the nuclear magnetic quantification peaks of the test substance, the standard substance, and the reference substance, a quantitative calculation formula for the test substance was established using the peak area of the reference substance as the reference, and the content of multiple batches of samples was tested and calculated. Result: Methodological studies showed that this method had a good linear relationship (r=0.999 8). The linear range was based on the ratio K [(potassium sorbate/reference DMSO quantitative characteristic peak area ratio)/(maleic acid/reference DMSO quantitative characteristic peak area ratio)], which was approximately 0.18-3.07. The precision RSD was 0.13%, and the repeatability RSD was 0.38%. Compared with the potassium sorbate content determination method recorded in the Chinese Pharmacopoeia (2020), the quantitative results of the two methods for multiple batches of samples were basically consistent. Conclusion: The established 1H qNMR method is easy to operate, requires a small amount of sample, and yields accurate results. It is suitable for situations where internal standards and samples are incompatible, as well as other application scenarios.
    • Bioassay
  • Simultaneous determination of added drugs in sleep-improving health food by HPLC-HRMS*
    YANG Hai-jiao, LI Meng-xuan, GUI Ying-qi, YANG Lu, ZHANG Xun, LI Zhi-yuan, HU Ting-ting
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1511-1522. https://doi.org/10.16155/j.0254-1793.2025-0249
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    Objective: To establish a qualitative and quantitative method for the simultaneous detection of 27 kinds of illegal sedative and hypnotic drugs, including imipramine hydrochloride, in sleep-improving health food products by high performance liquid chromatography-higt resolution mass spectrometry (HPLC-HRMS). Methods: :The samples were extracted with methanol solution by ultrasonic extraction. For samples containing oil, the extract was placed at -20 ℃ for 24 h, and the supernatant was filtered through a membrane. The HPLC-TOF/MS system was used for detection. Scanning was performed in both ESI positive and negative modes. The sample solution was separated by a five-fluorophenyl chromatographic column (100 mm×3.0 mm, 2.6 μm). In ESI positive mode, 0.1% formic acid water solution and 5 mmol · L-1 ammonium formate were used as the aqueous phase and acetonitrile as the organic phase. In ESI negative mode, water and 5 mmol · L-1 ammonium formate and acetonitrile were used as the mobile phases for gradient elution. Quantification was performed by the external standard method. The information of the exact mass numbers of the first and second levels, retention times, etc. of the 27 illegal additives was organized into a database, which can be used for qualitative screening and quantitative detection of these substances in unknown samples. Results: The linear relationship of the 27 sedative and hypnotic illegal additives in health food products was good within the linear range, with correlation coefficients (r) 0.999 5-0.999 9. The limit of detection (LOD) were 0.01-10 mg · kg-1, the limits of quantitation (LOQ) were 0.03-30 mg · kg-1, the average recovery rate was 70.4%-110.4%, and the RSD was 1.5%-8.0%. Conclusion: This method is simple in operation, highly sensitive and accurate, and can be used for high-throughput screening and confirmation of illegal drugs in various forms of sleep-improving health food products such as tablets, oral liquids and soft capsules.
  • Establishment of a method for determining aluminum residue in the fourth-generation IVIG separated by chromatography
    ZHANG Jun, DU Sheng-hua, LIANG Si-yuan, CHEN Fei, GOU Ting, LIN Tao, LIU Xun
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1523-1530. https://doi.org/10.16155/j.0254-1793.2025-0251
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    Objective: To establish a method for determining aluminum residue in the fourth-generation intravenous immunoglobulin (IVIG) separated by chromatography. Methods: :Atomic absorption spectrophotometry was employed, with an aluminum hollow cathode lamp as a narrow-line source. The aluminum residue in the fourth-generation IVIG was determined at a wavelength of 309.3 nm. Results: Under the conditions of this experiment, the specificity and accuracy were jointly evaluated. The spiked samples with three different concentrations showed the average recovery rates of 115.7%, 104.0%, and 100.3%. The established method showed the lower and upper quantitation limits of 3.003 2 μg · L-1 and 153.440 2 μg · L-1, respectively, with a good linear response to absorbance within this range (r≥0.999 0). The detection limit of the method was 0.991 1 μg · L-1. The relative standard deviation (RSD) of the intermediate precision verification results under different dates and personnel factors was 3.0%. The RSDs of the determination results at three different concentrations in the repeated experiment were 3.6%, 2.6%, and 3.2%. For the fourth-generation IVIG approved and marketed by our company, the average aluminum residue is approximately 10 μg · L-1. Resultsfrom long-term stability studies show an average of approximately 15 μg · L-1, while accelerated stability testing yields an average of approximately 20 μg · L-1. Conclusion: This method produces accurate and stable results, being suitable for the determination of aluminum residue in the fourth-generation IVIG.
    • Quality Control
  • Effects of white vaseline from different sources on the rheological properties and in vitro release of tacrolimus ointment*
    HOU Zhi-wen, ZOU Shi-tao, LI Shi-mei, HE Hai-bo, LIN Hua-qing, TANG Hai-ming
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1531-1540. https://doi.org/10.16155/j.0254-1793.2025-0272
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    Objective: To study the effects of white vaseline from different sources on the rheological properties and in vitro release of tacrolimus ointment. Methods: :Tacrolimus ointment was prepared with white vaseline from different sources. The rheological properties of white vaseline and ointment were observed by a rheometer. The in vitro release curves of the prepared tacrolimus ointment samples and reference preparation were determined by Franz diffusion cell method, and the rheological properties and in vitro release behavior were evaluated and analyzed. Results: All samples of white vaseline and tacrolimus ointment had shear thinning and solid-like rheological properties, presenting as pseudoplastic fluids. In the ointment samples of the same process and prescription, the rheological properties of white vaseline from different sources had positive correlations with the rheological properties of the corresponding ointment (P<0.001). The rheological properties of ointment had negative correlations with the in vitro release of the drug (P<0.05). Conclusion: The rheological properties and in vitro release rate of tacrolimus ointment are affected by white vaseline, which makes it possible to control the in vitro release rate of the ointment by changing white vaseline without changing the process and prescription. It provides a new idea for the development of generic drugs. In addition, the change of excipients is also a key factor affecting the quality of drugs.
  • In vitro release of indometacin gel
    XIE Li, CAO Jun-han, CHEN Hong, ZHENG Ping, LI Ping
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1541-1549. https://doi.org/10.16155/j.0254-1793.2025-0223
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    Objective: To establish a testing method for the in vitro release of indometacin gel and evaluate the batch-to-batch consistency and stability of the originator product, thus providing a scientific basis for generic drug development. Methods: :The Franz diffusion cell method was utilized. A 0.45 μm polyethersulfone microporous membrane was employed, with phosphate buffer (pH 6.0) as the receiving medium. Samples were fully collected at the 1st, 2nd, 3th, 4th, 5th, and 6th hours under conditions of constant stirring at 600 r · min-1 and a temperature maintained at (32±0.5) ℃. In compliance with the CDE draft guideline and USP <1724>, the release kinetic parameters of three batches of the originator product (at the initial time point, 0 month) and accelerated stability samples (after 3 months) were determined. Consistency and stability were evaluated based on the confidence intervals. Results: The established method demonstrated satisfactory membrane inertness, precision, discriminative power, and robustness. Significant batch-to-batch consistency was observed among the three batches of the originator product. The 90% confidence interval of the release rate ratio of the accelerated stability samples (after 3 months) to the initial samples (0 month) fell within the range of 90%-111%, indicating good stability. Conclusion: The established method is applicable for the testing and evaluation of the in vitro release of indometacin gel, offering valuable reference for generic drug development.
  • Study on the concentration of puerarin and icariin in Beagle dogs plasma by LC-MS/MS
    DONG Hui-juan, YANG Zhao-jun, PU Chang-bing, WANG Han-bin, CHEN Mo, WANG Lei, HAO Juan
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1550-1559. https://doi.org/10.16155/j.0254-1793.2025-0217
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    Objective: To establish a rapid and sensitive liquid chromatography-tandem mass spectrometry (LC-MS/MS) analysis method for determination of puerarin and icariin in Beagle dogs plasma following oral administration of Shenge Bushen capsules, and to investigate the toxicokinetics of its active components in Beagle dogs. The separation was carried out on a Kromasil C18 column (150 mm×2.1 mm, 5 µm) with the mobile phase consisting of 0.2% formic acid aqueous solution and 0.2% formic acid under gradient elution. ESI in positive ionization mode was performed to detect puerarin and icariin. Methods: :The analysis method was validated by investigating system applicability, selectivity and specificity, linearity and lower limit of quantification, precision and accuracy, matrix effect, carryover investigation, dilution precision and stability. The validated method was applied to a 39-week continuous administration of Beagle dogs toxicokinetic test to measure the concentrations of puerarin and icariin in the plasma and calculate the toxicokinetic parameters. Results: Under this method, there is no mutual interference between the analysis of puerarin and icariin and the internal standard. The quantitation ranges of puerarin and icariin were 2.0-500.0 ng · mL-1 and 1.0-250.0 ng · mL-1, respectively, with their LLOQ being 2.0 ng · mL-1 and 1.0 ng · mL-1, respectively. For plasma samples at low, mid, and high concentrations, the intra-batch and inter-batch precision RSD were<15%. No significant matrix effect or hemolytic matrix effect was detected, and carryover met the acceptance criteria. The RSD and RE for puerarin and icariin stability in plasma under short-term stability, freeze-thaw stability, long-term stability and autosampler stability were all≤15%. After the last dose. After consecutive 39-week dosing of Shenge Bushen capsules by gavage, the maximum concentrations (Cmax) of puerarin in Beagle dogs from the low, medium, and high dose groups were 2 574±1 514, 3 306±1 446, and 2 085±8 13.2 ng · mL-1, respectively. The Cmax of icariin in these groups were 14.51±18.01, 10.44±5.56, and 9.69±6.79 ng · mL-1, respectively. Four weeks after discontinuation of administration, both puerarin and icariin in plasma were eliminated from the body. Conclusion: The established LC-MS/MS method for the determining puerarin and icariin content in Beagle dogs plasma in this study is convenient, specific, and suitable for the determination of puerarin and icariin and toxicokinetic studies in Beagle dogs plasma.
    • Process Evaluation and Rapid Analysis
  • Optimization of the extraction process of total flavonoids from Artemisia Ordosica Krasch. root in Mongolian medicine*
    ZHANG Hong, LI Zhen, QIAO Xiang-dong, BAI Xian-xiang, XIAO Bin
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1560-1569. https://doi.org/10.16155/j.0254-1793.2025-0215
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    Objective: To maximize the yield of total flavonoids from Artemisia ordosica Krasch. root by optimizing the extraction process. Methods: :Based on single-factor experiments, the extraction process was optimized using a combined approach of the Box-Behnken response surface methodology and a back propagation (BP) neural network. The yield of total flavonoids was used as the index, with ethanol volume fraction, liquid-to-material ratio, and ultrasonication time as independent variables. Results: The total flavonoid yield optimized by BP neural network exceeds that achieved through the Box-Behnken response surface methodology. The optimal extraction conditions were an ethanol volume fraction of 72%, a liquid-to-material ratio of 42 ∶ 1, and an ultrasonication time of 90 min. Conclusion: The method is stable, reliable, and applicable for extracting total flavonoids from Artemisia ordosica Krasch. root.
  • An alternative method of rapid sterility testing in cell therapy products*
    MA Bing-cun, LIU Hua, LI Zeng-ting, LI Jing-yuan, CAO Qian-chao
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1570-1578. https://doi.org/10.16155/j.0254-1793.2025-0324
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    Objective: To investigate the equivalence of a rapid sterility testing method in cell therapy products with the sterility testing method outlined in the Pharmacopoeia of the Peoples Republic of China, providing insights for the validation of alternative sterility testing methods. Methods: :Following the guidelines of the General Principles 9201 Microbial Examination of Drugs in the Chinese Pharmacopoeia and other relevant technical guidance documents, statistical analysis techniques were employed to methodologically validate the rapid sterility testing method based on respiratory signal detection using the seven specified test strains in the Chinese Pharmacopoeia. Parameters such as method applicability, specificity, detection limit, reproducibility, and robustness were evaluated. Results: The rapid testing method utilized direct inoculation with a volume of 5 mL per bottle. The chi-square test for comparison of the rapid testing method with the pharmacopoeial method showed no significant difference in specificity, limit of detection, reproducibility, or robustness between the two methods under corresponding test conditions (P>0.05). The limit of detection of the rapid testing method was determined to be 1-2 cfu · mL-1. Under reproducibility test conditions, the detection time (to positive result reporting) fell within the range of 90% to 110% of the mean, except for Bacillus cereus with a 10-mL inoculum volume, where the detection time (57 h) did not meet the requirements. Conclusion: The rapid testing method based on automatic instrument monitoring offers advantages in terms of testing cycle, data integrity, and operational processes. It can replace the pharmacopoeial method for sterility testing of cell therapy products. Manufacturers are advised to adhere to the concept of quality by design, considering factors such as process control, production processes, sterility assurance levels, microbial contamination risks, and user benefit risks when formulating product release strategies.
  • Establishment and application of a method for detecting 19 psychotropic drugs in serum based on domestic LC-MS/MS
    LIU Feng, LUO Tian-yu, LIU Xiu
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1579-1586. https://doi.org/10.16155/j.0254-1793.2025-0122
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    Objective: To establish a rapid detection method for the concentrations of 19 psychotropic drugs in serum using domestic liquid chromatography-tandem mass spectrometry, and to study its application. Methods: :After obtaining the sample extract by precipitating proteins with organic reagents, the C18 chromatographic column was used for separation. The stable isotopes of each analyte were used as internal standards. The mobile phase was water and methanol, and gradient elution was carried out. The analysis was performed in the positive ion mode of the electrospray ionization source and the multiple reaction monitoring mode. Results: The detection limits of each analyte in this method range from 0.05 ng · mL-1 to 5.00 ng · mL-1, and the lower limits of quantification range from 0.206 ng · mL-1 to 20.0 ng · mL-1. The linear correlation coefficients of each analyte within the detection concentration range are good, with recovery rates ranging from 91.8% to 106.5%. The intra-day and inter-day precisions are both less than 10%, meeting the detection requirements. Research shows that there is no significant difference in the detection results between the domestic high-performance liquid chromatography tandem mass spectrometry detection system and the imported AB 4500MD system. Conclusion: This method features high sensitivity, high throughput and low economic cost. It aims to promote the application of domestic mass spectrometry instruments in therapeutic drug monitoring and provide a reference basis for drug concentration monitoring.
    • Metabolism Analysis
  • Establishment of the national standard materials for glucose in frozen human serum*
    YU Ting, SHEN Min, HU Ze-bin, HUANG Yan-jie
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1587-1592. https://doi.org/10.16155/j.0254-1793.2025-0129
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    Objective: To establish the national standard materials for glucose in frozen human serum for calibrating and evaluating the accuracy of serum glucose measurement methods. Methods: :Anticoagulant serum samples with clear appearance, free from obvious jaundice, lipids and hemolysis, and negative results for all four infectious diseases were selected. After three-stage filtration and sterilization, the samples were prepared into two levels of candidates. The assignment values of the candidates were based on WS/T 350-2011 reference procedure of the measurement of glucose in serum. The homogeneity, stability, and measurement uncertainty of the candidates were evaluated in accordance with the national metrological technical specification JJF 1343-2022 characterization, homogeneity, and stability assessment of reference materials. The commutability of the candidates was evaluated according to the WS/T 356-2024 guideline for evaluation of commutability of reference materials. Results: The homogeneity assay showed that the F values of candidates Ⅰ and Ⅱ were 1.355 3 and 1.473 3, respectively, which were less than F0.05 (1.511 7). Candidates Ⅰ and Ⅱ were stable for after storage for 6 h at 20-25 ℃, 2 days at 2-8 ℃,and at least 30 days at -20 ℃. The determined values of candidates Ⅰ and Ⅱ were (4.56±0.07) mmol · L-1 (k=2) and (6.60±0.10) mmol · L-1 (k=2), respectively. Candidates Ⅰ and Ⅱ demonstrated good commutability in six mainstream conventional detection systems. Conclusion: This batch of frozen serum glucose candidates excels in accuracy, uniformity, stability, and commutability and thus can be used as national standard materials for the calibration and accuracy verification of serum glucose measurement reagents. The findings are of significance for promoting the standardization and consistency of detection results.
  • Pharmacokinetic study and safety evaluation of human thrombin
    LI Yu-xing, LUO Guan-wen, HU Ji-jun, LIANG Zhao-hua, WANG Qi-qi, QIN Liang, ZHENG Yan
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1593-1605. https://doi.org/10.16155/j.0254-1793.2025-0092
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    Objective: To evaluate the pharmacokinetic characteristics and safety of human thrombin prepared from plasma, providing a scientific basis for clinical application. Methods: :For clinical indications such as capillary and small vein oozing with minor bleeding, where standard surgical techniques are ineffective or impractical for haemostasis, an animal model of liver resection surgery was used to study the pharmacokinetic characteristics of different doses of 125I-human thrombin in SD rats. For safety evaluation, human thrombin was applied to the skin or administered via intraperitoneal injection in New Zealand rabbits, and then whether the drug caused irritation to the skin or peritoneal cavity and the extent and reversibility of such irritation were observed. Results: Pharmacokinetic studies showed that after liver resection in SD rats, the radioactive concentration of 125I-human thrombin in plasma was extremely low and it was below the lower limit of quantification after 72 h. At 240 h post-administration, 125I-human thrombin was detected only in trace amounts in the liver (the site of administration), with concentrations below the limit of quantification in all other tissues and organs. Irritation study results showed that after continuous skin application of human thrombin at 1×10-1 mL · cm-2 for 7 days or a single intraperitoneal injection of 2 mL · kg-1 at a concentration of 1 000 IU · mL-1, mild irritation was observed at the damaged skin site in New Zealand rabbits, which showed a trend toward recovery after withdrawal. No obvious irritation was observed on intact skin or at the intraperitoneal site. Conclusion: Pharmacokinetic and safety evaluations indicate that following liver resection in rats, plasma drug concentrations were extremely low when human thrombin was applied topically, suggesting minimal systemic exposure and a low risk of thrombosis. In the rat model, human thrombin significantly reduced bleeding at the liver wound site within 5 min of administration, with a 100% survival rate at 24 h post-surgery. The skin and abdominal cavity irritation tests in New Zealand rabbits showed mild irritation on damaged skin, with no irritation on intact skin or the abdominal cavity, indicating high local application safety. Therefore, local application via spraying or in combination with gelatin sponges can be used for local auxiliary haemostasis in surgical or other mild to moderate bleeding wounds.
    • Safety Monitoring
  • Determination method for free protein content in group Bstreptococcus polysaccharide-protein conjugates*
    PU Li-zhen, KOU Ya-rong, SUN Wen-qian, LIU Piao, YANG Cheng-liang, WANG Hui-mei, TONG Xin
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1606-1615. https://doi.org/10.16155/j.0254-1793.2025-0023
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    Objective: To establish, verify and preliminarily apply the CE-LIF assay (capillary electrophoresis-laser induced fluorescence) for detecting the content of free carrier protein in polysaccharide-protein conjugates. Methods: :After pretreatment, the polysaccharide-protein conjugate was labeled with protein labeling solution and Chromeo P503 fluorescent reagent. After labeling, deionized water was added to terminate the reaction, and then the free carrier protein was detected by laser-induced fluorescence detector (LIF) after separation by micellar electrokinetic capillary chromatography. Methodological validation was also performed (specificity, detection limit and quantitation limit, linearity and range, intermediate precision, accuracy, solution stability, and robustness). Results: The method showed a good linear relationship between the amount of sample injected and the peak area in the concentration range of 0.05 to 20 μg · mL-1 of free protein, with coefficient of determination R2≥0.98; the RSD of precision were less than 5.0%; the recovery rate of the test samples was 108.1%, with an RSD of 8.1%; the detection limit concentration was 0.201 μg · mL-1. The quantitation limit concentration was 0.609 μg · mL-1. Capillary electrophoresis can well achieve the determination of free carrier protein in process samples, meeting the requirements of the pharmacopoeia (refer to the testing of the bulk conjugate of group A and group C meningococcal polysaccharide conjugate vaccine: the content of free carrier protein should not exceed 5%). Conclusion: The determination of free protein content in polysaccharide-protein conjugates has been established, with good linearity, accuracy, precision, and robustness, and the method can be applied to the quality control both of the multivalent GBS streptococcus and pneumococcal polysaccharide-tetanus toxoid conjugate vaccines in final products or bulks.
  • Content variations of four flavones and anti-cough effects of Citri Grandis Exocarpium of different aging years*
    TANG Yi, ZHOU Li-fen, HU Xiao-ling
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1616-1627. https://doi.org/10.16155/j.0254-1793.2024-1362
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    Objective: To compare the content of four flavones and anti-cough effects of decoction pieces and young fruits of different aging years of Citri Grandis Exocarpium. Methods: :High performance liquid chromatography was employed to measure the content of four flavones in the decoction pieces and young fruits of different aging years of Citri Grandis Exocarpium. Compounds were separated on ELite 31113003 Supersil ODS column (200 mm×4.6 mm, 25 μm), mobile phase was 0.1% formic acid solution (A)-0.1% methyl alcohol solution (B) for gradient elution (0~10 min,30%B→60%B; 10~25 min, 60%B→75%B; 25~32 min, 75%B→100%B; 32~35 min, 100%B→30%B), the column temperature was set at 30 ℃, the flow rate was 1 mL · min-1,the detected wavelength was 283 nm, the injection volume was 10 μL. Ammonia water was used to induce cough in mice, which were then treated with the decoction pieces and young fruits of different aging years. The cough incubation period and cough frequency in 3 min were recorded. Results: The content of naringin, naringenin, and nobiletin in decoction pieces showed an overall decreasing trend, while that of hesperetin kept increasing with the increase in aging years. As the aging years increased, the content of naringin and naringenin in young fruits showed an overall decreasing trend, while that of hesperetin and nobiletin presented large fluctuations. Compared with the blank group, the decoction pieces aged for 0, 1, and 2 years and young fruits of all aging years prolonged the cough incubation period (P<0.01) and reduced the cough frequency in 3 min (P<0.01). There was no significant difference in cough incubation period or cough frequency among the blank group and decoction pieces aged for 3 and 4 years. Conclusion: All decoction pieces and young fruits tested in this study meet the criteria for total flavone content and naringin content in the Pharmacopoeia of the People’s Republic of China (2020 edition) and local standards (2017 edition) in Guangdong Province. The decoction pieces aged for 0, 1, and 2 years and young fruits of all aging years have good anti-cough effect.
  • Simultaneous determination of 11 phytoestrogens in three substrates based on HPLC-MS/MS
    XU Wen-jia, ZHANG Xiao-meng, ZHANG Hai-fang, LI Jia-hui, FU Ce-yi, LIANG Ying, CHEN Lu
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1628-1636. https://doi.org/10.16155/j.0254-1793.2024-1316
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    Objective: To establish an HPLC-MS/MS method for the determination of 11 phytoestrogens (calycosin-7-O-β-D-glucopyranoside, secolsolariciresinol diglucoside, genisitn, hesperidin, quercetin genistein, puerarin, liquiritin, daidzein, formononetin, biochaninA) in three substrates. Methods: :The analytes were separated on a Capcellcorl C18 (150 mm×4.6 mm, 2.7 μm) with the mobile phases of methanol and 0.1%(v/v) formic acid aqueous solution with gradient elution. The flow rate was 0.3 mL · min-1, and the column temperature was 30 ℃.The electrospray ionization source with positive ion mode and negative ion mode was used for analyzing the 11 phytoestrogens in the multiple reaction monitoring (MRM) mode. Results: Good separation for 11 compounds were obtained under the optimized chromatographic conditions, the calibration curves for 11 compounds were liner and the correlation coefficients were above 0.999 in the concentration ranges of the investigation. The recoveries of 11 compounds ranged from 90.2%-104.7% (for liquid), 90.4%-105.1% (for emulsion) and 90.9%-102.4% (for gel). The relative standard deviations (RSDs) were less than 5.5%. Conclusion: The method is accurate, sensitive and effective, which could be used for the quality control phytoestrogens in three substrates.
  • Quantitative detection of AB-38b in brain tissue of SD rats based on a highly sensitive LC-MS/MS method
    SHA Pian, PAN Dan-dan, GU Zhu-lin, QIN Ya-wei
    Chinese Journal of Pharmaceutical Analysis. 2025, 45(9): 1637-1645. https://doi.org/10.16155/j.0254-1793.2025-0269
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    Objective: To develop and validate a highly sensitive analytical method that can quantitatively measure the concentration of AB-38b in normal rat brain tissue and reveal the pharmacokinetics of AB-38b in rat brain tissue. Methods: :Tolvaptan was selected as the internal standard (IS). Brain tissue samples were pretreated with methanol for protein precipitation. Liquid chromatography was performed with a Shim-pack VP-ODS C18 column (2.0 mm×150 mm,5 μm), mobile phase A of ammonium acetate, mobile phase B of methanol, a flow rate of 0.2 mL · min-1, a column temperature of 40 ℃, an auto-sampler temperature of 4 ℃, and an injection volume of 5 µL. The ionization mode was electrospray ionization (ESI), and multiple reaction monitoring (MRM) positive ion mode was used to detect AB-38b (m/z 705.2→618.3) and tolvaptan (m/z 449.3→252.2). Comprehensive methodological validation was conducted for this method, including establishment of the standard curve and the lower limit of quantification, residual effect investigation, accuracy and precision verification, matrix effect exploration, and determination of extraction recovery rates. Thirty male SD rats (240±14 g) were randomly assigned into 5 groups, with 6 rats in each group. After 12 h of fasting but free access to water, they were administrated with AB-38b at a single oral dose of 50 mg · kg-1. At the time points of 0, 15, 50, 90, and 480 min post-administration, the rats were weighed and sacrificed via the carbon dioxide method. The brain tissue was collected and weighed, and tissue homogenates were prepared with phosphate buffer. After processing according to the tissue sample treatment method, the concentrations of AB-38b in rat brain tissue samples were determined by LC-MS/MS. Results: The linear range of AB-38b was 2.5-150 ng · mL-1 (R2>0.999), and the lower limit of quantitation was 2.5 ng · mL-1. The intra-day precision and inter-day accuracy were 88.54%-104.56% and 95.24%-102.31%, respectively. The precision (RSD) was less than 9%. The extraction recovery of AB-38b and IS in rat brain homogenate samples was 81.9%-95.9%, RSD<15%. The matrix effect range of AB-38 b was 87.74%-96.21%, RSD<15%. The residual peak area at the retention time of AB-38b was less than 20% of the peak area of LLOQ, and the residual peak area at the retention time of internal standard was less than 5% of the peak area. AB-38b was stable in brain tissue homogenate at room temperature for 6 h, three freeze-thaw cycles, 24 h in the sampler, and long-term (-80 ℃ ) storage for 60 days, with RSD<12.7%. The results suggested that accuracy and precision, extraction recovery, matrix effect, residual effect, and stability all met the acceptance criteria. Conclusion: The LC-MS/MS method established in this study is rapid, sensitive, and specific, and can accurately determine the content of AB-38b in rat brain tissue.
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