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100721-27-5

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100721-27-5 Usage

Check Digit Verification of cas no

The CAS Registry Mumber 100721-27-5 includes 9 digits separated into 3 groups by hyphens. The first part of the number,starting from the left, has 6 digits, 1,0,0,7,2 and 1 respectively; the second part has 2 digits, 2 and 7 respectively.
Calculate Digit Verification of CAS Registry Number 100721-27:
(8*1)+(7*0)+(6*0)+(5*7)+(4*2)+(3*1)+(2*2)+(1*7)=65
65 % 10 = 5
So 100721-27-5 is a valid CAS Registry Number.

100721-27-5Downstream Products

100721-27-5Relevant academic research and scientific papers

Site-Specific Immuno-PET Tracer to Image PD-L1

Wissler, Haley L.,Ehlerding, Emily B.,Lyu, Zhigang,Zhao, Yue,Zhang, Si,Eshraghi, Anisa,Buuh, Zakey Yusuf,McGuth, Jeffrey C.,Guan, Yifu,Engle, Jonathan W.,Bartlett, Sarah J.,Voelz, Vincent A.,Cai, Weibo,Wang, Rongsheng E.

, p. 2028 - 2036 (2019)

The rapid ascension of immune checkpoint blockade treatments has placed an emphasis on the need for viable, robust, and noninvasive imaging methods for immune checkpoint proteins, which could be of diagnostic value. Immunoconjugate-based positron emission tomography (immuno-PET) allows for sensitive and quantitative imaging of target levels and has promising potential for the noninvasive evaluation of immune checkpoint proteins. However, the advancement of immuno-PET is currently limited by available imaging tools, which heavily rely on full-length IgGs with Fc-mediated effects and are heterogeneous mixtures upon random conjugation with chelators for imaging. Herein, we have developed a site-specific αPD-L1 Fab conjugate with the chelator 1,4,7-triazacyclononane-N,N′,N″-triacetic acid (NOTA), enabling radiolabeling for PET imaging, using the amber suppression-mediated genetic incorporation of unnatural amino acid (UAA), p-azidophenylalanine. This Fab conjugate is homogeneous and demonstrated tight binding toward the PD-L1 antigen in vitro. The radiolabeled version, 64Cu-NOTA-αPD-L1, has been employed in PET imaging to allow for effective visualization and mapping of the biodistribution of PD-L1 in two normal mouse models, including the capturing of different PD-L1 expression levels in the spleens of the different mouse types. Follow-up in vivo blocking studies and ex vivo fluorescent staining further validated specific tissue uptakes of the imaging agent. This approach illustrates the utility of UAA-based site-specific Fab conjugation as a general strategy for making sensitive PET imaging probes, which could facilitate the elucidation of the roles of a wide variety of immune checkpoint proteins in immunotherapy.

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