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Transcript
Sensitive analysis and isolation of ROR1+ B cells
for research on chronic lymphocytic leukemia
Introduction
is provided in an unconjugated form, without toxic
preservatives or endotoxins. Figure 1 shows a typical
immunophenotyping experiment with a CLL sample.
PBMCs were labeled with a panel of eight MACS® Antibodies
and analyzed by flow cytometry using the following setup:
violet laser (405 nm): CD20-VioBlue®; blue laser (488 nm):
CD43-FITC, CD5-PE, CD79b-PerCP-Vio700™, CD19-PE-Vio770™;
red laser (633 nm): Anti-ROR1-APC, CD3-APC-Vio770.
10³
10²
10²
10¹
1
0
-1
10¹
10⁰
10¹
10²
10¹
1
0
-1
-1 0 1
10³
10³
10³
10²
10²
10¹
1
0
-1
-1 0 1
10¹
10²
1
0
-1
-1 0 1
10³
10³
10¹
10²
10³
Anti-ROR1-APC
10³
CD19-PE-Vio770
10³
CD19-PE-Vio770
10²
10¹
CD79b-PerCP-Vio700
Tools for the analysis and isolation
of ROR1+ B cells from CLL samples
10¹
CD43-FITC
CD5-PE
CD5-PE
CD20-VioBlue
ROR1 as a B cell marker in CLL research
ROR1 is a member of the receptor tyrosine kinase–like
orphan receptor (ROR) family and has characteristics of
an oncofetal antigen. ROR1 signaling increases cell survival
via the wnt pathway ¹. The protein is expressed on B cells
from CLL blood samples, but not from blood of healthy
donors.¹,²,³ ROR1 is also expressed on various solid tumors ⁴,
but not in major adult tissues apart from low levels in
adipose tissue, on embryonic stem cells, and transiently at
an early stage of B cell development⁵. Therefore, ROR1 is
a potential marker to identify and isolate CLL B cells from
blood samples for downstream analysis.
10²
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1
0
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-1 0 1
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CD3-APC-Vio770
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1
0
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-1 0 1
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10²
10³
CD5-PE
Figure 1: Identification of ROR1+ cells and other immune cells in
PBMCs from a CLL sample. Cells were labeled with CD20-VioBlue,
CD43-FITC, CD5-PE, CD79b-PerCP-Vio700, CD19-PE-Vio770, Anti-ROR1APC, and CD3-APC-Vio770, and analyzed on the MACSQuant Analyzer
10. CD19+ROR1+ B cells are shown in magenta, CD19+ROR1– B cells in light
blue, T cells in yellow, and NK cells in black.
Analysis of ROR1 B cells in CLL samples
Miltenyi Biotec offers an Anti-ROR1 antibody, which
increases sensitivity and specificity of flow cytometric
B cell analysis in CLL research. It is available as a conjugate
with PE, APC, or biotin. For functional studies, the antibody
+
Sensitive analysis and isolation of ROR1+ B cells | March 2014
10³
CD5-PE
CD5-PE
The challenge of analyzing lymphoid cells in chronic
lymphocytic leukemia research
Flow cytometric analysis of lymphoid cells from chronic
lymphocytic leukemia (CLL) samples requires a complex
panel of multiple markers. Most of these markers are
expressed on both normal and malignant cells, and only
characteristic marker expression profiles help distinguish
between normal and malignant cells. Identification of new
markers and the optimization of antibody panels for flow
cytometric immunophenotyping would greatly enhance
leukemia research.
Analysis of malignant B cells becomes especially difficult
with samples containing only very low amounts of these
cells, e.g., in minimal residual disease (MRD). Enrichment of
malignant B cells from these samples would help overcome
this obstacle. However, current techniques for the isolation
of B cells do not allow for a distinction between malignant
and normal cells. This drawback hampers the analysis of
differential gene expression, for example.
1
Copyright © 2014 Miltenyi Biotec GmbH. All rights reserved.
Conclusion
Isolation of ROR1+ cells from CLL samples
For the isolation of ROR1+ B cells, Miltenyi Biotec has
developed the Anti-ROR1 MicroBead Kit. Using this kit,
ROR1+ cells are indirectly magnetically labeled with an
Anti-ROR1-PE antibody and Anti-PE MicroBeads.
Subsequently, the labeled ROR1+ cells are isolated manually
using LS or MS Columns, or automatically with the
autoMACS® Pro Separator. The isolated ROR1+ B cells are
then ready for any downstream analysis. ROR1+ cells can
be enriched to high purities and numbers suitable for
further research processing – even from samples with
very low ROR1+ cell frequencies, e.g., in MRD (fig. 2).
A
B
10³
3.15%
10²
CD19-APC
CD19-APC
8.15%
10¹
1
0
-1 88.58%
-1 0 1
10²
0.82%
10³
10²
CD19-APC
CD19-APC
10²
10¹
10²
10³
CD19-APC
CD19-APCCD19-APC
10³
93.86%
10¹
0.25%
10¹
0.09%
10¹
10²
10³
Anti-ROR1-PE
Positive fraction
10²
1
0
-1 3.01%
-1 0 1
0.09%
10¹
Positive fraction
2.89%
10³
10²
Anti-ROR1-PE
10³
1.33%
1
0
-1 98.49%
-1 0 1
0.09%
10¹
10²
Negative fraction
10³
0.81%
1
0
-1 90.37%
-1 0 1
0.00%
10¹
Anti-ROR1-PE
Negative fraction
8.72%
1. Fukuda, T. et al. (2008) Antisera induced by infusions of autologous
Ad-CD154-leukemia B cells identify ROR1 as an oncofetal antigen and
receptor for Wnt5a. Proc. Acad. Natl. Sci USA 105: 3047–3052.
2. Baskar, S. et al. (2012) Targeting malignant B cells with an immunotoxin
against ROR1. MAbs 4: 349–361.
3. Baskar, S. et al. (2008) Unique cell surface expression of receptor
tyrosinase kinase ROR1 in human B-cell chronic lymphocytic leukemia.
Clin. Cancer Res. 14: 396–404.
4. Zhang, S. et al. (2012) The onco-embryonic antigen ROR1 is expressed
by a variety of human cancers. Am. J. Pathol. 181: 1903–1910.
5. Hudecek, M. et al. (2010) The B-cell tumor–associated antigen ROR1
can be targeted with T cells modified to express a ROR1-specific chimeric
antigen receptor. Blood 116: 4532–4541.
10¹
Anti-ROR1-PE
10³
References
4.63%
1
0
-1 94.55%
-1 0 1
0.12%
10¹
Anti-ROR1 antibodies enhance the sensitivity and
specificity of flow cytometric immunophenotyping
of CLL samples.
Anti-ROR1 antibodies allow the identification and
enumeration of B cells for CLL research.
The Anti-ROR1 MicroBead Kit enables the enrichment
of ROR1+ CLL B cells – even from samples containing
only very low amounts of these cells, for example,
in MRD.
Isolation of ROR1+ cell populations to high purities
facilitates research on the specific features and
functions of CLL B cells.
Original fraction
Original fraction
10³
•
•
•
•
10²
10³
Anti-ROR1-PE
Anti-ROR1-PE
1.15%
97.96%
10²
MACS Product*
Order no.
Anti-ROR1-PE, human
130-098-317
Anti-ROR1-APC, human
130-098-320
Anti-ROR1-Biotin, human
130-098-312
Anti-ROR1 pure, human
130-098-243
Anti-ROR1 MicroBead Kit, human
130-103-929
MACSQuant Analyzer 10
130-096-343
autoMACS Pro Separator – Starter Kit
130-092-545
* Products are for research use only.
10¹
1
0
-1 0.80%
-1 0 1
Miltenyi Biotec’s portfolio comprises thousands
of antibodies. Select the antigen and conjugate you
need at www.miltenyibiotec.com/antibodies
0.09%
10¹
10²
10³
Anti-ROR1-PE
Miltenyi Biotec’s Custom Antibody Design Service
enables you to tailor single and multicolor antibody
conjugates, as well as multicolor antibody panels
that perfectly meet your specific research needs.
Learn more about it at
www.miltenyibiotec.com/customantibodies
Figure 2: Enrichment of ROR1 cells from PBMCs of a donor with
MRD. ROR1+ cells were isolated using the Anti-ROR1 MicroBead
Kit, either manually (A) or automatically using the autoMACS Pro
Separator (B). Cells were fluorescently labeled with Anti-ROR1-PE and
CD19-APC and analyzed by flow cytometry. Purities of the manually
and automatically isolated cells amounted to 94% and 98%, and yields
amounted to 45% and 97%, respectively.
+
For more information on the principle of
MACS MicroBead Technology, see
www.miltenyibiotec.com/microbead
Miltenyi Biotec provides products and services worldwide. Visit www.miltenyibiotec.com/local to find your nearest Miltenyi Biotec contact.
Unless otherwise specifically indicated, Miltenyi Biotec products and services are for research use only and not for therapeutic or diagnostic use.
MACS, the MACS logo, Vio, VioBlue, Vio700, and Vio770 are registered trademarks or trademarks of Miltenyi Biotec GmbH.
Copyright © 2014 Miltenyi Biotec GmbH. All rights reserved.
Sensitive analysis and isolation of ROR1+ B cells | March 2014
2
Copyright © 2014 Miltenyi Biotec GmbH. All rights reserved.