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- SIGMA
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- G1145-10g
- 2025年08月20日
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- 详细信息
- 文献和实验
- 技术资料
- 保存条件:
常温
- 保质期:
根据瓶身LOT号查询
- 英文名:
Glass beads, acid-washed
- 库存:
有现货
- 供应商:
浙江羽翔生物科技有限公司
- CAS号:
见瓶身
- 规格:
10G
属性
粒径
150-212 μm (70-100 U.S. sieve)
应用
- 酵母菌落分解,用于酵母双杂交筛选
- 娄地青霉(Penicillium roqueforti)菌丝样本的DNA提取
- 破碎嗜热链球菌(Streptococcus thermophilus)和德氏乳杆菌保加利亚亚种(Lactobacillus delbrueckii subsp. Bulgaricus ),以测定酶活性
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文献和实验Mass Spectrometry Proteotyping-Based Detection and Identification of Staphylococcus aureus, Escherichia coli, and Candida albicans in Blood.
Bloodstream infections (BSIs), the presence of microorganisms in blood, are potentially serious conditions that can quickly develop into sepsis and life-threatening situations. When assessing proper treatment, rapid diagnosis is the key; besides clinical judgement performed by attending physicians, supporting microbiological tests typically are performed, often requiring microbial isolation and culturing steps, which increases the time required for confirming positive cases of BSI. The additional waiting time forces physicians to prescribe broad-spectrum antibiotics and empirically based treatments, before determining the precise cause of the disease. Thus, alternative and more rapid cultivation-independent methods are needed to improve clinical diagnostics, supporting prompt and accurate treatment and reducing the development of antibiotic resistance. In this study, a culture-independent workflow for pathogen detection and identification in blood samples was developed, using peptide biomarkers and applying bottom-up proteomics analyses, i.e., so-called "proteotyping". To demonstrate the feasibility of detection of blood infectious pathogens, using proteotyping, Escherichia coli and Staphylococcus aureus were included in the study, as the most prominent bacterial causes of bacteremia and sepsis, as well as Candida albicans, one of the most prominent causes of fungemia. Model systems including spiked negative blood samples, as well as positive blood cultures, without further culturing steps, were investigated. Furthermore, an experiment designed to determine the incubation time needed for correct identification of the infectious pathogens in blood cultures was performed. The results for the spiked negative blood samples showed that proteotyping was 100- to 1,000-fold more sensitive, in comparison with the MALDI-TOF MS-based approach. Furthermore, in the analyses of ten positive blood cultures each of E. coli and S. aureus, both the MALDI-TOF MS-based and proteotyping approaches were successful in the identification of E. coli, although only proteotyping could identify S. aureus correctly in all samples. Compared with the MALDI-TOF MS-based approaches, shotgun proteotyping demonstrated higher sensitivity and accuracy, and required significantly shorter incubation time before detection and identification of the correct pathogen could be accomplished.
Evaluating Modulators of “Regulator of G‐protein Signaling” (RGS) Proteins
RGS Protein Modulators with the Transcreener GDP Assay and a Rate‐Modified Gα Subunit Materials Compound library (e.g., Sigma LOPAC
【求助】最近在做hsv tk,所用前药为粉末状GCV(购自sigma),但不知道怎么溶解
qulinyd 最近在做hsv tk,所用前药为粉末状GCV(购自sigma),但不知道怎么溶解合适,还请各位帮帮忙哦 freecell 你从sigma买来的东西,应该有个datasheet吧: Preparation Instructions Soluble at 10 mg/ml in 0.1 N HCl. Storage/Stability Store desiccated
不贵,因为我们老板比较小气,所以在买药品方面比较慎重。在用玻璃珠的那种方法中,其它药品都齐了,就差玻璃珠了。谢谢!答3:告诉你一种简便实用的提取酵母质粒的方法,其纯度完全可以用来测序和做PCR。你可以尝试一下。氯化苄提取真菌基因组的方法。在1.5ml Appendorf管中加入0.1g菌体和500ul提取液,振荡使之充分混合,再加入10%SDS100ul,氯化苄300ul,剧烈振荡,使管内混合物成乳状。50度保温1h,每隔10min振荡混合一次,然后加入300ul 3mol/LNaCl(ph=
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