新型柱前衍生试剂分析草甘膦的高效液相色谱研究

以2,5-二甲氧基苯磺酰氯(DMOSC)为柱前衍生化试剂,建立了柱前衍生草甘膦的紫外检测反相高效液相色谱法,并优化了衍生化条件,得最佳条件:衍生温度35℃,时间15 min,pH 10.0,草甘膦与DMOSC的摩尔比为1∶6。HPLC分析条件:采用Kromasil C18柱,流速1.0 mL/min,柱温30℃,检测波长220 nm,流动相为甲醇-乙腈-磷酸盐缓冲溶液(0.02 mol/L、pH 5.5),三者的体积比为15∶5∶80。结果表明:草甘膦质量浓度在5~100μg/mL范围内线性关系良好,相关系数为0.996 2,检测限为0.067μg/mL。实验表明该方法反应条件温和,灵敏度高,衍生产物稳定。     

柱前衍生反相高效液相色谱法测定绞股蓝茶叶中17种游离氨基酸含量

建立2,4-二硝基氟苯柱前衍生化-反相高效液相色谱法测定绞股蓝茶叶中17种游离氨基酸的含量。以Phenomenex Gemini NX C18(4.6mm×250mm,5μm)为分析柱,采用梯度洗脱,流动相A为0.05mol·L-1乙酸钠(pH=6.4,含0.1%N,N-二甲基甲酰胺),流动相B为乙腈-水(1∶1,v/v),检测波长为360nm,柱温35℃;经方法学考察,该方法具有良好的稳定性和重现性。测定结果表明,绞股蓝茶叶中17种游离氨基酸总量为39.79mg·g-1,其中人体必需氨基酸占游离氨基酸总量的36.57%。从氨基酸含量考虑,绞股蓝茶叶具备一定的开发利用价值。     

HPLC-MS/MS法快速测定人血浆中美利曲辛及生物等效性研究

目的:建立测定人血浆中关利曲辛浓度的高效液相串联质谱法(HPLC-MS/MS),用于氟哌噻吨美利曲辛片的生物等效性研究.方法:以Agilent ZORBAX Eclipse Plus C18(4.6mm× 150mm,5μm)为色谱柱,流动相为乙腈(含1%甲酸):0.02mo·L-1甲酸铵水溶液(80∶20,V∶),流速:0.8mL·min-1;柱温:40℃,以醋酸乙酯:二氯甲烷(4∶1,V∶V)为提取剂.样品经电喷雾离子源正离子化后,通过三重四级杆串联质谱仪,采用选择反应监测(SRM)对美利曲辛(m/z 292.2→232.2)和阿米替林(m/z 278.1-91.0)进行测定.结果:美利曲辛的高(50μg·L-1)、中(20μg·L-1)、低(0.5μg·L-1)3个浓度的平均回收率分别为97.53%、104.03%和106.87%,日内(n=5)、日间(n=3)RSD均小于15%;分析方法的最低定量限为0.2μg·L-1.线性范围为:0.2～60μg·L-1,回归方程为:F=1.8691ρ+0.0555,r=0.9986(n=9),权重为1/ρ2.结论:该方法灵敏、准确、简单、快速,可用于临床血浓监测和药动学研究.     

高效液相色谱法测定黄瓜皮中绿原酸含量

目的:建立高效液相色谱法测定黄瓜皮中绿原酸含量的方法.方法:采用Zorbax Eclipse XDB-C18色谱柱(150 ×4.6 nm,5 μm);流动相:甲醇- 0.4%磷酸溶液(25∶75);流速:1.0 ml·min-1;检测波长:326nm;柱温:30℃.结果:绿原酸的线性范围为0.0111～0.1332 ...     

高效液相色谱法测定肌肽滴眼液中L-肌肽的含量及有关物质

目的:建立肌肤滴眼液中L-肌肤的含量测定的HPLC方法.方法:采用Kromasil NH2色谱柱(200 mm × 4.6mm,5 μm),流动相为乙腈-40 mmol·L-1磷酸氢二钾溶液(44:56,磷酸调pH 6.3).流速1.0 mL·min-1,检测波长为210 ml,柱温为35℃.结果:肌肤在9.93～99.3μg·mL-1范围内线性关系良好(r=0.999 8),平均回收率为99.8%(RSD=1.0%,n=9),滴眼液中含L-肌肽的标示百分含量为97.0%～102.0%.结论:该方法操作简便、重复性好、专属性强,可用作肌肤滴眼液中L-肌肽的质量控制.     

2种HPLC-柱后衍生化-荧光检测法测定远志中黄曲霉毒素的比较

对远志中测定黄曲霉毒素的2种柱后衍生化方法(碘衍生化和光化学衍生化)进行分析比较。样品经过免疫亲和柱净化，HPLC-柱后衍生化-荧光检测器检测；采用C₁₈(250 mm×4.6 mm,5μm)色谱柱，荧光检测。柱后衍生化系统：(1)碘衍生化法，以甲醇-乙腈-水(25∶20∶55)为流动相；衍生溶液为0.05%碘溶液，流速为0.3 m L·min^-1，衍生反应温度为70℃；(2)光化学衍生化法，以甲醇-乙腈-水(35∶15∶50)为流动相。碘衍生化方法中，黄曲霉毒素B₂、G₂在3.8～19 pg范围内线性关系良好，B₁在10.4～52 pg范围内线性关系良好，G₁在10.8～54 pg范围内线性关系良好；在光化学衍生化方法中，黄曲霉毒素B₂、G₂在1.9～45.6 pg范围内线性关系良好，B₁在5.2～124.8 pg范围内线性关系良好，G₁在5.4～129.6 pg范围...     

柱前衍生化HPLC同时测定霍山石斛中13种游离氨基酸含量

为建立柱前衍生化HPLC同时测定霍山石斛中13种游离氨基酸的方法。采用Waters XBridge C_(18)色谱柱(250 mm×4. 6 mm,5μm);流动相为0. 1 mol/L醋酸钠缓冲液-乙腈∶水(4∶1),梯度洗脱;流速1. 0 mL/min,柱温35℃;检测波长254 nm。在该色谱条件下霍山石斛中13种游离氨基酸分离较好,平均加样回收率为92. 7%~104. 3%,RSD 2. 5%。该方法简便、准确、重现性好,适用于霍山石斛中13种游离氨基酸的同时测定。     

HPLC同时测定伤科黄水中6个生物碱的含量

建立HPLC同时测定伤科黄水中6个生物碱的方法。采用XBridge C₁₈色谱柱(3. 5μm,2. 1 mm×100 mm),柱温35℃,测定波长280 nm,以0. 1%磷酸溶液(每100 mL加0. 3 g十二烷基苯磺酸钠)(A)-乙腈-水-磷酸-十二烷基苯磺酸钠(90∶10∶0. 1∶0. 3)(B)为流动相,进行梯度洗脱(0～30 min,B%:35～70; 30～31 min,B%:70～35; 31～40min,B%:35)。经方法学验证,黄柏碱、药根碱、表小檗碱、黄连碱、巴马汀、小檗碱等共6个生物碱分离情况良好,在测定时间段内无明显干扰峰;加样回收率均在95%～115%之间,RSD%均小于5%;精密度RSD%均小于5%;在测定浓度范围内(1～50μg/mL)线性关系良好,相关系数(R^2)大于0. 999。3个不同批次供试品的测定结果较一致。本研究建立的HPLC分析方法可用于同时测定伤科黄水中6个生物碱的含量。     

柱前衍生HPLC法测定大鼠血浆中的河蚌糖胺聚糖

目的:建立柱前衍生高效液相色谱法(HPLC)用于河蚌糖胺聚糖在大鼠血浆中的含量测定。方法:使用异硫氰酸荧光素(FITC)对河蚌糖胺聚糖进行荧光标记,色谱柱为Shodex SB-804HQ(8.0×300 mm),流动相为流速为0.5 m L·min-1的0.1 mol·L-1的Na H2PO4-Na2HPO4缓冲液(p H 7.8),柱温30℃,激发波长495 nm,发射波长520 nm。结果:FITC对河蚌糖胺聚糖的荧光标记率为70;线性范围为5~120μg·m L-1,批内和批间精密度均小于15.0%,提取回收率为51.5~58.6%,样品在血浆中稳定性良好。结论:血浆中内源性杂质不干扰样品的测定,建立的方法符合生物样本的分析要求。     

高效液相色谱法测定降糖1号胶囊中淫羊藿苷的含量

目的:建立测定降糖1号胶囊中淫羊藿苷含量的方法。方法:室温条件下超声提取降糖1号胶囊中的淫羊藿苷,用D101大孔吸附树脂柱纯化提取物,高效液相色谱法(HPLC)测定含量,色谱柱:Hypersil ODS2(4.6mm×200mm,5μm);流动相:乙腈-水(30:70);流速:1ml/min,检测波长270nm;柱温:30℃。结果:淫羊藿苷的进样量在0.08μg-0.28μg范围内线性关系良好(r=0.9999),平均加样回收率(n=6)为96.66%,RSD为2.14%。结论:该方法简便、准确、重复性好,可用于降糖1号胶囊的质量控制。     

Gabapentin hybrid peptides and bioconjugates

Synthetic approaches to gabapentin bioconjugates that overcome the tendency of gabapentin to cyclize into its γ-lactam are studied. Gabapentin was converted by N-acylation at its N-terminus into di-, tri-, and tetrapeptides (l-Ala-Gbp, l-Val-Gbp, l-Ala-l-Phe-Gbp, Gly-l-Ala-β-Ala-Gbp). Carboxyl-activated Boc-protected gabapentin was used to N-, O-, and S-acylate small peptides and hormones to give conjugates that could also provide prodrugs containing conformationally constrained gabapentin units.     

Investigating Gabapentin Polymorphism Using Solid-State NMR Spectroscopy

Solid-state NMR spectroscopy (SSNMR), coupled with powder X-ray diffraction (PXRD), was used to identify the physical forms of gabapentin in samples prepared by recrystallization, spray drying, dehydration, and milling. Four different crystalline forms of gabapentin were observed: form I, a monohydrate, form II, the most stable at ambient conditions, form III, produced by either recrystallization or milling, and an isomorphous desolvate produced from desolvating the monohydrate. As-received gabapentin (form II) was ball-milled for 45 min in both the presence and absence of hydroxypropylcellulose (HPC). The samples were then stored for 2 days at 50°C under 0% relative humidity and analyzed by ¹³C SSNMR and PXRD. High-performance liquid chromatography was run on the samples to determine the amount of degradation product formed before and after storage. The ¹H T ₁ values measured for the sample varied from 130 s for the as-received unstressed material without HPC to 11 s for the material that had been ball-milled in the presence of HPC. Samples with longer ¹H T ₁ values were substantially more stable than samples that had shorter T ₁ values. Samples milled with HPC had detectable form III crystals as well. These results suggest that SSNMR can be used to predict gabapentin stability in formulated products.     

加巴喷丁与卡马西平治疗坐骨神经痛的疗效比较

目的 探讨加巴喷丁与卡马西平治疗坐骨神经痛的临床疗效.方法 选取2017年1月 ～2020年1月治疗的坐骨神经痛患者80例,随机分为观察组和对照组各40例,观察组给予加巴喷丁治疗,对照组给予卡马西平治疗.采用视觉模拟评分法(VAS)对两组患者治疗前、治疗4周后的疼痛程度进行评估,采用生活质量量表(QOL)评价两组患者治...     

Synthesis and biological evaluation of conformationally restricted Gabapentin analogues.

A series of conformationally restricted Gabapentin analogues has been synthesised. The pyrrolidine analogue (R)-2-Aza-spiro[4.5]decane-4-carboxylic acid hydrochloride (3a) had an IC50 of 120 nM, similar to that of Gabapentin (IC50 = 140 nM), at the Gabapentin binding site on the alpha2delta subunit of a calcium channel. Compound (3a) also reversed carrageenan induced hyperalgesia in rats.     

Role of Branched-Chain Aminotransferase Isoenzymes and Gabapentin in Neurotransmitter Metabolism

Abstract: Because it is well known that excess branched-chain amino acids (BCAAs) have a profound influence on neurological function, studies were conducted to determine the impact of BCAAs on neuronal and astrocytic metabolism and on trafficking between neurons and astrocytes. The first step in the metabolism of BCAAs is transamination with α-ketoglutarate to form the branched-chain α-keto acids (BCKAs). The brain is unique in that it expresses two separate branched-chain aminotransferase (BCAT) isoenzymes. One is the common peripheral form [mitochondrial (BCATm)], and the other [cytosolic (BCATc)] is unique to cerebral tissue, placenta, and ovaries. Therefore, attempts were made to define the isoenzymes' spatial distribution and whether they might play separate metabolic roles. Studies were conducted on primary rat brain cell cultures enriched in either astroglia or neurons. The data show that over time BCATm becomes the predominant isoenzyme in astrocyte cultures and that BCATc is prominent in early neuronal cultures. The data also show that gabapentin, a structural analogue of leucine with anticonvulsant properties, is a competitive inhibitor of BCATc but that it does not inhibit BCATm. Metabolic studies indicated that BCAAs promote the efflux of glutamine from astrocytes and that gabapentin can replace leucine as an exchange substrate. Studying astrocyte-enriched cultures in the presence of [U-¹⁴C]glutamate we found that BCKAs, but not BCAAs, stimulate glutamate transamination to α-ketoglutarate and thus irreversible decarboxylation of glutamate to pyruvate and lactate, thereby promoting glutamate oxidative breakdown. Oxidation of glutamate appeared to be largely dependent on the presence of an α-keto acid acceptor for transamination in astrocyte cultures and independent of astrocytic glutamate dehydrogenase activity. The data are discussed in terms of a putative BCAA/BCKA shuttle, where BCATs and BCAAs provide the amino group for glutamate synthesis from α-ketoglutarate via BCATm in astrocytes and thereby promote glutamine transfer to neurons, whereas BCATc reaminates the amino acids in neurons for another cycle.     

The Stabilizing Effect of Moisture on the Solid-State Degradation of Gabapentin

Gabapentin is known to undergo intramolecular cyclization to form a lactam (gaba-l) with concomitant loss of water. Gabapentin was milled in a planetary mill for 15–60 min. Unmilled and milled gabapentin were stored at 50°C with relative humidity ranged between 5% and 90%. The unmilled and milled samples were assayed for gabapentin and gaba-l by reversed phase-high-performance liquid chromatography and also subjected to powder X-ray diffraction, solid-state nuclear magnetic resonance and surface area analyses. The rates of lactamization in the milled gabapentin samples correlated to increased surface area, milling duration, and in-process lactam levels. This effect of milling could not be explained solely by the increase in surface area with increased milling time but was more likely due to increased regions of crystal disorder caused by the mechanical and thermal milling stresses. The lactamization rate of milled gabapentin samples was greatest in the presence of the lowest humidity conditions and dramatically decreased with increasing humidity. In particular, milled gabapentin appeared to be much more stable at humidity levels greater than 31% RH. This finding could not be attributed to the possibility of lactam hydrolysis at high humidity but rather to a competitive annealing process wherein milling-induced crystal defects were lost upon exposure to atmospheric moisture thereby stabilizing the milling-damaged drug substance.     

Combination Therapy of Gabapentin and N-Acetylcysteine Against Posttraumatic Epilepsy in Rats

Traumatic brain injury (TBI) is a major public health problem worldwide that is associated with increased mortality and morbidity. Posttraumatic epilepsy (PTE) is one of the sequelae of TBI. The aim of this study was to investigate the role of N-acetylcysteine (NAC) as an adjuvant on the efficacy of levetiracetam (LEV) and gabapentin (GBP) in PTE model encouraged by pentylenetetrazol (PTZ) after mild-TBI in male Sprague–Dawley rats. Mild-TBI was performed by the weight-drop method in male Sprague–Dawley rats. PTE model was developed by injecting PTZ (30+15+15 mg/kg, 30 min intervals, i.p.) 7 days after head trauma. After the development of posttraumatic seizures, the rats were treated with NAC (100 mg/kg), LEV (50 mg/kg), GBP (100 mg/kg), NAC+LEV and NAC+GBP intraperitoneally for 14 days. Seizures related to PTE were scored by video-EEG recording. Motor performance of the animals was also evaluated in the rotarod test. 50 mg/kg LEV and 100 mg/kg GBP reduced seizures related to PTE. LEV alone (p?=?0.009), but the administration of GBP+NAC (p?=?0.015) was more effective on PTE-related seizure control. However, GBP+NAC application adversely affected the fall latency in the rotarod test. In terms of trauma-related seizure control, there was no statistically significant difference between the use of prophylactic LEV and symptomatic LEV. LEV alone or the combination of GBP with NAC provides more effective seizure control in the PTE facilitated by PTZ. On the other hand, the use of prophylactic LEV did not have any extra effect on posttraumatic seizure development and control.

     

Gabapentin Administration Reduces Reactive Gliosis and Neurodegeneration after Pilocarpine-Induced Status Epilepticus

The lithium-pilocarpine model of epilepsy reproduces in rodents several features of human temporal lobe epilepsy, by inducing an acute status epilepticus (SE) followed by a latency period. It has been proposed that the neuronal network reorganization that occurs during latency determines the subsequent appearance of spontaneous recurrent seizures. The aim of this study was to evaluate neuronal and glial responses during the latency period that follows SE. Given the potential role of astrocytes in the post-SE network reorganization, through the secretion of synaptogenic molecules such as thrombospondins, we also studied the effect of treatment with the α2δ1 thrombospondin receptor antagonist gabapentin. Adult male Wistar rats received 3 mEq/kg LiCl, and 20 h later 30 mg/kg pilocarpine. Once SE was achieved, seizures were stopped with 20 mg/kg diazepam. Animals then received 400 mg/kg/day gabapentin or saline for either 4 or 14 days. In vitro experiments were performed in dissociated mixed hippocampal cell culture exposed to glutamate, and subsequently treated with gabapentin or vehicle. During the latency period, the hippocampus and pyriform cortex of SE-animals presented a profuse reactive astrogliosis, with increased GFAP and nestin expression. Gliosis intensity was dependent on the Racine stage attained by the animals and peaked 15 days after SE. Microglia was also reactive after SE, and followed the same pattern. Neuronal degeneration was present in SE-animals, and also depended on the Racine stage and the SE duration. Polysialic-acid NCAM (PSA-NCAM) expression was increased in hippocampal CA-1 and dentate gyrus of SE-animals. Gabapentin treatment was able to reduce reactive gliosis, decrease neuronal loss and normalize PSA-NCAM staining in hippocampal CA-1. In vitro, gabapentin treatment partially prevented the dendritic loss and reactive gliosis caused by glutamate excitotoxicity. Our results show that gabapentin treatment during the latency period after SE protects neurons and normalizes PSA-NCAM probably by direct interaction with neurons and glia.