| 查看: 853 | 回复: 1 | |||
| 本帖产生 1 个 MolEPI ,点击这里进行查看 | |||
gloomy6159铁杆木虫 (职业作家)
|
[求助]
蛋白质检测方法 修正的洛瑞法 请问谁有?
|
||
| 修正的洛瑞即可以同时测定蛋白质和腐殖质含量的方法 最好是很详细的 谢谢 |
回复此楼» 收录本帖的淘帖专辑推荐
 【分子生物】EPI帖 |
» 本帖@通知
» 猜你喜欢
筑牢营养安全线:以精准检测,护健康基石
已经有0人回复
-
推荐一些20种氨基酸检测的实际应用案例
已经有0人回复
-
化学工程及工业化学论文润色/翻译怎么收费?
已经有85人回复
-
不合理蛙科研实验中的趣事:实验器材的 “乌龙”
已经有0人回复
-
不合理蛙科研实验中的趣事:和实验材料的 “斗智斗勇”
已经有0人回复
-
蛋白质检测:精准分析,解锁生物分子的密码
已经有0人回复
-
不合理蛙科研实验之小鼠实验:严谨设计,解析生命机制的重要载体
已经有0人回复
-
不合理蛙科研实验之重金属检测:精准筛查,守护健康与环境的防线
已经有0人回复
-
不合理蛙科研实验之“蛙测重金属我背锅三千”
已经有0人回复
-
不合理蛙科研实验之“鼠逃三次我发三篇SCI”
已经有0人回复
» 本主题相关价值贴推荐,对您同样有帮助:
- 求蛋白质相互作用研究方法...
已经有12人回复
- 急求:得到蛋白质后,想对其进行二级结构的检测,求方法和机构
已经有9人回复
- 关于蛋白质检测方法可以向那些SCI杂志投稿?
已经有4人回复
- 【求助/交流】请问做蛋白质消化用考马斯亮蓝法还是福林-酚法检测好?
已经有5人回复
- 【求助】【急】请问有谁做过细胞核STR分型检测和线粒体DNA测序?急求详细方法!
已经有15人回复
- 【求助】AOAC 的蛋白质、脂肪、水分和灰分的测定方法
已经有8人回复
- 【求助/交流】BSA法测蛋白质浓度的原理和方法
已经有19人回复
- 【求助】请问检测重金属离子的方法有哪些?
已经有18人回复
- 【原创】蛋白质快速测定方法步骤
已经有5人回复
- 【求助】蛋白质含量的测定都有哪几种方法,适用情况以及优缺点。
已经有10人回复
blackrose8089
铁杆木虫 (职业作家)
- MolEPI: 16
- 应助: 100 (初中生)
- 贵宾: 0.11
- 金币: 10636.6
- 散金: 155
- 红花: 30
- 沙发: 6
- 帖子: 3702
- 在线: 790.1小时
- 虫号: 614948
- 注册: 2008-09-28
- 专业: 植物学研究的新技术、新方
【答案】应助回帖
★ ★ ★ ★ ★ ★ ★ ★ ★
西瓜(金币+4): Good! 2011-12-03 22:24:16
gloomy6159(金币+50): 可以留下联系方式吗?有问题想问下啊 2011-12-06 14:02:06
wanhscn(金币+5, MolEPI+1): Good!授予专家指数! 2011-12-06 14:41:16
西瓜(金币+4): Good! 2011-12-03 22:24:16
gloomy6159(金币+50): 可以留下联系方式吗?有问题想问下啊 2011-12-06 14:02:06
wanhscn(金币+5, MolEPI+1): Good!授予专家指数! 2011-12-06 14:41:16
|
楼主看是下面这个不? http://www.ruf.rice.edu/~bioslabs/methods/protein/lowry.html Hartree-Lowry and Modified Lowry Protein Assays Considerations for use The Lowry assay (1951) is an often-cited general use protein assay. For some time it was the method of choice for accurate protein determination for cell fractions, chromatography fractions, enzyme preparations, and so on. The bicinchoninic acid (BCA) assay is based on the same princple and can be done in one step, therefore it has been suggested (Stoscheck, 1990) that the 2-step Lowry method is outdated. However, the modified Lowry is done entirely at room temperature. The Hartree version of the Lowry assay, a more recent modification that uses fewer reagents, improves the sensitivity with some proteins, is less likely to be incompatible with some salt solutions, provides a more linear response, and is less likely to become saturated. The Hartree-Lowry assay will be described first. Principle Under alkaline conditions the divalent copper ion forms a complex with peptide bonds in which it is reduced to a monovalent ion. Monovalent copper ion and the radical groups of tyrosine, tryptophan, and cysteine react with Folin reagent to produce an unstable product that becomes reduced to molybdenum/tungsten blue. Equipment In addition to standard liquid handling supplies a spectrophotometer with infrared lamp and filter is required. Glass or polystyrene (cheap) cuvettes may be used. Procedure - Hartree-Lowry assay Reagents Reagent A consists of 2 gm sodium potassium tartrate x 4 H20, 100 gm sodium carbonate, 500 ml 1N NaOH, H20 to one liter (that is, 7mM Na-K tartrate, 0.81M sodium carbonate, 0.5N NaOH final concentration). Keeps 2 to 3 months. Reagent B consists of 2 gm sodium potassium tartrate x 4 H20, 1 gm copper sulfate (CuSO4 x 5H20), 90 ml H20, 10 ml 1N NaOH (final concentrations 70 mM Na-K tartrate, 40 mM copper sulfate). Keeps 2 to 3 months. Reagent C consists of 1 vol Folin-Ciocalteau reagent diluted with 15 vols water. Assay Prepare a series of dilutions of 0.3 mg/ml bovine serum albumin in the same buffer containing the unknowns, to give concentrations of 30 to 150 micrograms/ml (0.03 to 0.15 mg/ml). Add 1.0 ml each dilution of standard, protein-containing unknown, or buffer (for the reference) to 0.90 ml reagent A in separate test tubes and mix. Incubate the tubes 10 min in a 50 degrees C bath, then cool to room temperature. Add 0.1 ml reagent B to each tube, mix, incubate 10 min at room temperature. Rapidly add 3 ml reagent C to each tube, mix, incubate 10 min in the 50 degree bath, and cool to room temperature. Final assay volume is 5 ml. Measure absorbance at 650 nm in 1 cm cuvettes. Analysis Prepare a standard curve of absorbance versus micrograms protein (or vice versa), and determine amounts from the curve. Determine concentrations of original samples from the amount protein, volume/sample, and dilution factor, if any. Procedure - modified Lowry (room temperature) Reagents Dissolve 20 gm sodium carbonate in 260 ml water, 0.4 gm cupric sulfate (5x hydrated) in 20 ml water, and 0.2 gm sodium potassium tartrate in 20 ml water. Mix all three solutions to prepare the copper reagent. Prepare 100 ml of a 1% solution (1 gm/100 ml) of sodium dodecyl sulfate (SDS). Prepare a 1 M solution of NaOH (4 gm/100 ml). For the 2x Lowry concentrate mix 3 parts copper reagent with 1 part SDS and 1 part NaOH. Solution is stable for 2-3 weeks. Warm the solution to 37 degrees C if a white precipitate forms, and discard if there is a black precipitate. Better, keep the three stock solutions, and mix just before use. Prepare 0.2 N Folin reagent by mixing 10 ml 2 N Folin reagent with 90 ml water. Kept in an amber bottle, the dilution is stable for several months. Assay Dilute samples to an estimated 0.025-0.25 mg/ml with buffer. If the concentration can't be estimated it is advisable to prepare a range of 2-3 dilutions spanning an order of magnitude. Prepare 400 microliters each dilution. Duplicate or triplicate samples are recommended. Prepare a reference of 400 microliters buffer. Prepare standards from 0.25 mg/ml bovine serum albumin by adding 40-400 microliters to 13 x 100 mm tubes + buffer to bring volume to 400 microliters/tube. Add 400 microliters of 2x Lowry concentrate, mix thoroughly, incubate at room temp. 10 min. Add 200 microliters 0.2 N Folin reagent very quickly, and vortex immediately. Complete mixing of the reagent must be accomplished quickly to avoid decomposition of the reagent before it reacts with protein. Incubate for 30 min. more at room temperature. Use glass or polystyrene cuvettes to read the absorbances at 750 nm. If the absorbances are too high, they may be read at 500 nn. Comments Recording of absorbances need only be done within 10 min. of each other for this modified procedure, whereas the original Lowry required precise timing of readings due to color instability. This modification is less sensitive to interfering agents and is more sensitive to protein than the original. As with most assays, the Lowry can be scaled up for larger cuvette sizes, however more protein is consumed. Proteins with an abnormally high or low percentage of tyrosine, tryptophan, or cysteine residues will give high or low errors, respectively. References Lowry, OH, NJ Rosbrough, AL Farr, and RJ Randall. J. Biol. Chem. 193: 265. 1951. Oostra, GM, NS Mathewson, and GN Catravas. Anal. Biochem. 89: 31. 1978. Stoscheck, CM. Quantitation of Protein. Methods in Enzymology 182: 50-69 (1990). Hartree, EF. Anal Biochem 48: 422-427 (1972). |
2楼2011-12-03 20:04:26