top
Please input keywords
Database
ニュース&PR
お問い合わせ
JP
CN
EN
KR
About us
会社情報
私たちの歩み
管理スタッフ
企業文化
社会的責任
共に働く
Antibody Assets
Project Integrum
Antibody discovery platforms
Pipeline
Clinical pipeline
Preclinical pipeline
RenMice
RenMab
RenLite
RenNano
動物・細胞モデル
Pharmacology service
ゲノム編集
研究提携
IR
Stock Information
Financial Reports
Listing Documents
Announcements & Notices
Corporate Governance
Investor Calendar
Email Alert
IR Contact
Order
*Country
日本
アメリカ
中国
オーストラリア
シンガポール
イギリス
フランス
ドイツ
スイス
イタリア
カナダ
韓国
オランダ
ベルギー
スウェーデン
その他
*Province
*City
*Name
*Telephone
*Company
*Position
*Email
*Verification code
*Verification Code
Home
動物・細胞モデル
動物・細胞モデル
Tumor cell lines
Humanized cell lines
Text
B-hPD-L1 plus/hPCSK9 MC38
Common name
 		B-hPD-L1 plus/hPCSK9 MC38 Catalog number    220215
Aliases CD274, PDCD1L1

FH3, FHCL3, HCHOLA3, LDLCQ1, 

NARC-1, NARC1, PC9

Disease  Colon carcinoma
Organism
 		Mouse 
 		Strain  C57BL/6
Tissue types Colon Tissue  Colon
Description 

The mouse Pd-l1 gene and Pcsk9 gene were replaced by human PD-L1 and PCSK9 coding sequence in B-hPD-L1 plus/hPCSK9 MC38 cells. Human PD-L1 and human PCSK9 is highly expressed in  B-hPD-L1 plus/hPCSK9 MC38.

Application

B-hPD-L1 plus/hPCSK9 MC38 cells have the capability to establish tumors in vivo and can be used for efficacy studies.

Targeting strategy

Gene targeting strategy for B-hPD-L1 plus/hPCSK9 MC38 cells. The exogenous promoter and human PD-L1 coding sequence was inserted to replace partial exon 3 of mouse Pd-l1 gene. The insertion disrupts the endogenous murine Pd-l1 gene, resulting in a non-functional transcript. The exogenous promoter and human PCSK9 coding sequence was inserted to replace part of murine exons 1-3. The insertion disrupts the endogenous murine Pcsk9 gene, resulting in a non-functional transcript.

Protein expression analysis 

from clipboard


PD-L1 and PCSK9 expression analysis in B-hPD-L1 plus/hPCSK9 MC38 cells. Single cell suspensions from wild-type MC38 and B-hPD-L1 plus/hPCSK9 MC38 cultures were stained with species-specific anti-PD-L1 antibody. Human PD-L1 was detected on the surface of B-hPD-L1 plus/hPCSK9 MC38 cells but not wild-type MC38 cells. Human PCSK9 was detected by ELISA in B-hPD-L1 plus/hPCSK9 MC38 cells but not wild-type MC38 cells. The 1-D07 clone of B-hPD-L1 plus/hPCSK9 MC38 cells was used for in vivo experiments.

Tumor growth curve & Body weight changes

from clipboard


Subcutaneous homograft tumor growth of B-hPD-L1 plus/hPCSK9 MC38 cells. B-hPD-L1 plus/hPCSK9 MC38 cells (5x105) and wild-type MC38 cells (5x105) were subcutaneously implanted into C57BL/6N mice (female, 7-week-old, n=6). Tumor volume and body weight were measured twice a week. (A) Average tumor volume ± SEM. (B)  Body weight (Mean± SEM). Volume was expressed in mm3 using the formula: V=0.5 X long diameter X short diameter2. As shown in panel A, B-hPD-L1 plus/hPCSK9 MC38 cells were able to establish tumors in vivo and can be used for efficacy studies.

Protein expression analysis 

from clipboard

PD-L1 and PCSK9 expression analysis in B-hPD-L1 plus/hPCSK9 MC38 cells. B-hPD-L1 plus/hPCSK9 MC38 cells were subcutaneously transplanted into C57BL/6 mice (n=6), and on 32 days post inoculation, tumor cells were harvested and assessed for human PD-L1 and human PCSK9 expression. As shown, human PD-L1 was highly expressed on the surface of tumor cells and human PCSK9 was secreted in large quantities. Therefore, B-hPD-L1 plus/hPCSK9 MC38 cells can be used for in vivo efficacy studies.




+86-010-56967680
info@bbctg.com.cn
Copyright © 2021 Biocytogen. All Rights Reserved
Powered by Fractal-technology