Moxi Flow instrument with USB power cord, US style USB power adapter, and Type MF-S cassette pack

Application Notes

Brochures

Protocols

Quick Start Guides

Software Downloads

Technical Notes

User Manuals

Customer Data

Product Videos

Reagents

Assays

Accessories

Antibodies

Cassettes

Instruments

• Overview 
•   
  • Specifications 
  •   
    • How It Works 
    •   < style="padding:0px;overflow:visible !important;display:inline;" >Customer Data
       

Moxi Flow is a fully automated, cassette-based flow cytometer that combines unparalleled ease of use with the precision and accuracy normally only associated with more expensive flow cytometers. This ultra-small instrument uses patented microfluidic thin-film cassettes that enable automatic load and measure operation. The Moxi Flow is also the only flow cytometer that auto-aligns the laser to each cassette to enable highly repeatable and robust results every time. No PMT gain adjustment is required. No warm up time required. Just insert a cassette, pipette your sample, and read the results in 10 seconds.

Select from one of our standard applications (i.e., Cell Counts, Viability, Apoptosis) or run the system in open “2 Parameter Flow Cytometry” mode for the ultimate in assay flexibility. This miniature open platform can be used for your most common cell assay needs, or to develop sophisticated, custom assays right at your fingertips.

Moxi Flow generates data using the industry standard FCS 3.1 format so you can open and analyze your results using your ORFLO’s VESTIGO software (coming soon), or any other standardized flow cytometry analysis software. Data is transferred simply and easily to a PC or MAC using a mini-USB cable and the on board “USB-on-the-Go” functionality. No additional software is required to perform the data transfer.

• Cell Count with >95% accuracy
• Viability with PI
• Apoptosis with Annexin V
• Precise cell/particle (Coulter Principle)
• Blood analysis (RBC counts, WBC counts, CD4 counts, etc.)
• Somatic Cell Counts in Milk

Below are screen shots taken directly from the Moxi Flow. The left screen shot is a scatter plot of fluorescence intensity of the Propidium Iodide (PI), used to select for dead cells, versus cell volume on the x axis, converted to cell diameter. The middle screen shot is cell volume only, which shows the cell volume heterogeneity of the cancer line population along with subtle shift in the mean cell volume of the dead cell population. The right screen shot shows the fluorescence intensity of the baseline viable cell population versus the dead cell population.

Propidium Iodide was used to detect the exact cell count of the dead, non viable cells. The viability percent is displayed in the yellow text box. The concentration and volume of the viable live cells and non viable cells is displayed in the black text boxes.

Below are screen shots taken directly from the Moxi Flow. The left screen shot is a scatter plot of fluorescence intensity of the Annexin V PE versus cell volume on the x axis, converted to cell diameter. The right screen shot is cell volume only, which shows the cell volume heterogeneity of the cancer line population. Annexin V conjugated with PE was used to detect the exact number of cancer cells that were apoptotic. The percent of apoptotic cells is displayed in the yellow text box. The concentration and volume of the non-apoptotic and apoptotic cells is displayed in the black text boxes. This together with the above cell viability and cell count tests gives a read of over all cell health.

Below are screen shots taken directly from the Moxi Flow. The left screen shot is a scatter plot of fluorescence intensity of the RFP (tdTomato, DS Red, Nile Red, etc.) versus cell volume on the x axis, converted to cell diameter. The right screen shot is fluorescence only, which shows heterogeneity the transfect RFP within the cancer line population. The RFP in this case was tdTomato. In this example there were two distinct populations of the transfected cell lines. Both are * positively transfected. It is possible that this could be an inidication of cell cycle, the lower population could be in G0/G1 phase with approximay half the DNA of the upper population, G2/M phase.

In all tests shown in the figures below Tonbo PE conjugated flow cytometery antibodies were used.

In the screen shots below the PBMC sample was screened for the number of CD2 positive versus CD2 negative cells, using Tonbo’s PE Anti Human CD2 antibody (RPA-2.10).

The RPA-2.10 antibody reacts with human CD2, an approximay 50 kDa glycoprotein, and a member of the Ig superfamily. CD2, also known as LFA-2, is a receptor for CD58 in the human and is expressed on the cell surface of 80-90% of human peripheral blood lymphocytes, a subset of NK cells, and all mature T cells. CD2 mediates lymphocyte adhesion and is involved in T cell activation. RPA-2.10 is reported to block mixed lymphocyte reaction. Please choose the appropriate format for each application.

The Moxi Flow Flow Cytometer Cell Counter (Coulter Principle based) is able to clearly separate out the CD2 positive cells versus the CD2 negative cells, delivering a highly accurate and precise count of the two populations. The fold difference between the positive and negative white blood cells is a simple relative protein quantitation method.

In the screen shots below the PBMC sample was screened for the number of CD3 positive versus CD3 negative cells, using Tonbo’s PE Anti Human CD3 antibody (Hit3a).

The Hit3a antibody is specific for human CD3e, also known as CD3 epsilon, a 20 kDa subunit of the T cell receptor complex, along with CD3 gamma and CD3 delta. These integral membrane protein chains assemble with additional chains of the T cell receptor (TCR), as well as CD3 zeta chain, to form the T cell receptor – CD3 complex. Together with co-receptors CD4 or CD8, the complex serves to recognize antigens bound to MHC molecules on antigen-presenting cells. These interactions promote T cell receptor signaling (T cell activation), inducing cell proliferation, differentiation, production of cytokines or activation-induced cell death. CD3 is differentially expressed during thymocyte-to-T cell development and on all mature T cells.

The Hit3a antibody is a widely used phenotypic marker for human T cells. In addition, binding/cross-linking of Hit3a antibody to CD3e can induce cell activation. The antibody has also been demonstrated to be cross-reactive with Chimpanzee CD3. Please choose the appropriate format for each application.

The Moxi Flow Flow Cytometer Cell Counter (Coulter Principle based) is able to clearly separate out the CD3 positive white blood cells versus the CD3 negative white blood cells, delivering a highly accurate and precise count of the two populations. The fold difference between the positive and negative white blood cells is a simple relative protein quantitation method.

In the screen shots below the PBMC sample was screened for the number of CD4 positive (t cells) versus CD4 negative cells, using Tonbo’s PE Anti Human CD4 antibody (OKT4).

The OKT4 antibody reacts with human CD4, a 59 kDa protein which acts as a co-receptor for the T cell receptor (TCR) in its interaction with MHC Class II molecules on antigen-presenting cells. The extracellular domain of CD4 binds to the beta-2 domain of MHC Class II, while its cytoplasmic tail provides a binding site for the tyrosine kinase lck, facilitating the signaling cascade that initiates T cell activation. CD4, and co-receptors CCR5 and CXCR4, may also be utilized by HIV-1 to enter T cells. Human CD4 is typically expressed on thymocytes, some mature T cell populations such as Th17 and T regulatory (Treg) cells, as well as on dendritic cells. The OKT4 antibody is widely used as a phenotypic marker for CD4 expression. It is cross-reactive with CD4 in several non-human species, including Chimpanzee, Cynomolgus and Rhesus. This antibody recognizes a different epitope, and thus does not block binding of, the alternative Anti-Human CD4 antibody clone RPA-T4 (Reinherz EL, et al. 1979. Proc. Natl. Acad. Sci. 76:4061-4065)

The Moxi Flow Flow Cytometer Cell Counter (Coulter Principle based) is able to clearly separate out the CD4 positive white blood cells versus the CD4 negative white blood cells, delivering a highly accurate and precise count of the two populations. The fold difference between the positive and negative white blood cells is a simple relative protein quantitation method.

In the screen shots below the PBMC sample was screened for the number of CD8 positive versus CD4 negative cells, using Tonbo’s PE Anti Human CD8 antibody (SK1).

The SK1 antibody is specific for the 32-34 kDa alpha chain of human CD8, known as CD8a or CD8 alpha. CD8a can form a homodimer (CD8 alpha-alpha), but is more commonly expressed as a heterodimer with a second chain known as CD8b or CD8 beta. CD8 acts as a co-receptor for antigen recognition and subsequent T cell activation that is initiated upon binding of the T cell receptor (TCR) to antigen-bearing MHC Class I molecules. The cytoplasmic domains of CD8 provide binding sites for the tyrosine kinase lck, facilitating intracellular signaling events that lead to T cell activation, development, and cytotoxic effector functions. CD8+ cytotoxic T cells (CTLs) play an important role in inducing cell death of tumor cells, as well as cells infected by virus, bacteria or parasites.

The SK1 antibody is widely used as a phenotypic marker for CD8 on cytotoxic T cells, thymocytes, as well as on certain cell types that do not also express the TCR, including some NK cells and lymphoid dendritic cells. It is cross-reactive with CD8 in several non-human species, including Baboon, Chimpanzee, Cynomolgus and Rhesus. If used together with an alternative Anti-Human CD8a clone, RPA-T8, the SK1 antibody will not block binding of RPA-T8 to CD8a.

The Moxi Flow Flow Cytometer Cell Counter (Coulter Principle based) is able to clearly separate out the CD8 positive white blood cells versus the CD8 negative white blood cells, delivering a highly accurate and precise count of the two populations. The fold difference between the positive and negative white blood cells is a simple relative protein quantitation method.

In the screen shots below the PBMC sample was screened for the number of CD11 positive versus CD11 negative cells, using Tonbo’s PE Anti Human CD8 antibody (ICRF44).

The ICRF44 antibody reacts with human CD11b, also known as integrin alpha M. This 165-170 kDa cell surface glycoprotein is part of a family of integrin receptors that mediate adhesion between cells (cell-cell) and components of the extracellular matrix, e.g. fibrinogen (cell-matrix). In addition, integrins are active signaling receptors which recruit leukocytes to inflammatory sites and promote cell activation. Complete, functional integrin receptors consist of distinct combinations of integrin chains which are differentially expressed. Integrin alpha M (CD11b) assembles with Integrin beta-2 (CD18) into a receptor known as Macrophage Antigen-1 (Mac-1) or complement receptor type 3 (CR3). This receptor binds and induces intracellular signaling through ICAM-1, ICAM-2, ICAM-3 and ICAM-4 on endothelial cells and can also facilitate removal of iC3b bearing foreign cells.

The ICRF44 antibody is widely used as a marker for CD11b expression on macrophages, granulocytes, and subsets of NK cells. It is reported to be cross-reactive with a number of non-human species including Baboon, Chimpanzee, Cynomolgus, Rhesus and Swine.

The Moxi Flow Flow Cytometer Cell Counter (Coulter Principle based) is able to clearly separate out the CD11 positive white blood cells versus the CD11 negative white blood cells, delivering a highly accurate and precise count of the two populations. The fold difference between the positive and negative white blood cells is a simple relative protein quantitation method.

In the screen shots below the PBMC sample was screened for the number of CD19 positive b cells versus CD19 negative white blood cells, using Tonbo’s PE Anti Human CD19 antibody (SJ25C1).

The SJ25C1 antibody reacts with human CD19, a 95 kDa glycoprotein which acts as a co-receptor, along with CD21 (CR2), CD81 (TAPA-1) and CD225 (Leu13), in support of the functional B cell receptor (BCR). This complex provides antigen-specific recognition and subsequent activation of B cells to proliferate and differentiate into antibody-secreting cells (plasma cells) or memory B cells, which are crucial for secondary antigen encounter. Upon activation and tyrosine phosphorylation, the CD19 molecule can provide an anchor for cytoplasmic signaling proteins such as GRB2, SOS or PLCG2. CD19 is a lineage-differentiation marker, as its expression is detectable at the earliest B cell stages, through development, and is finally lost upon transition to mature plasma cells.

The SJ25C1 antibody is widely used as a phenotypic marker for CD19 expression on B cells, as well as on dendritic cell subsets.

The Moxi Flow Flow Cytometer Cell Counter (Coulter Principle based) is able to clearly separate out the CD19 positive white blood b cells versus the CD19 negative white blood cells, delivering a highly accurate and precise count of the two populations. The fold difference between the positive and negative white blood cells is a simple relative protein quantitation method.

Moxi GO 532nm laser (MXG001)
1 PMT - 561nm/LP filter (e.g. PE, PI) - US Version
Moxi GO 488nm laser (MXG002)
1 PMT - User-swappable 525/45nm (e.g. FITC, GFP) or 561nm/LP (PE,PI) filters
Moxi GO II 488nm laser (MXG102)
2 PMT system 525/45nm (e.g. FITC, GFP) and 561nm/LP (PE, PI)

Add To Wish List

Request Info

Application Notes

Brochures

Protocols

Quick Start Guides

Software Downloads

Technical Notes

User Manuals

Product Videos

Reagents

Assays

Accessories

Antibodies

Cassettes

• Overview 
•   
  • Specifications 
  •   < style="padding:0px;overflow:visible !important;display:inline;" >How It Works
     

Increase the pace of scientific discovery with ORFLO’s next generation Moxi Go™ or Moxi Go II™ Next Gen Flow Cytometers. With a one (Moxi GO) or two (Moxi GO II) fluorescent channels, swappable filter sets (MXG002 - Moxi GO 488nm), configurable laser the Moxi Go can be designed to meet your labs cell analysis needs.  Every assay also delivers simultaneous cell count & volume determination, using single-use flow cell.  This eliminates the hassle of traditional flow associated with cleaning, maintenance, clearing of clogs, cross contamination and occasionally replacement of bottles and tubes.  

Furthermore the Moxi Go™ or Moxi Go II™ use very little sample volume, 75ul's allowing you to conserver precious, expensive sample, such as stem cells.  Cell concentrations as low as 10,000 cells per ml are possible, which most experiments would enable a little as 5ul's of sample diluted in 70ul's of PBS.

The Moxi Go™ or Moxi Go II™ can be utilized as an assay development instrument and many powerful cell based assays can easily be optimized and run on the system.  These include:

• Cell surface immuno-labeling
• In-Cell Protein Quant
• CRISPR/Transfection Optimization Studies
• Up to 4 plex bead based ELISA's using our new on board MPX Relative Quantitation Ap
• In cell Wester Blots
• Reactive Oxidation Species Experiments
• Calein AM studies
• Phagocytosis Analysis
• Mito Potential Experiements

The Moxi Go™ or Moxi Go II™ come standard with an ultra-intuitive, plug-and-play interface with free OS updates as long as you own the instrument. No prior flow cytometry experience is required you simply just plug and play.

Product Code: MXA005

MOXI Z System Check Beads (5 mL)

Sh List

Related Products

Accessories

Cassettes

Instruments

• Specifications

Product Code: MXA006

Moxi Z Diluent, 100 mL

Related Products

Reagents

Accessories

Cassettes

Instruments

• Specifications

Product Code: MXA009

Moxi Z Diluent,  5 mL

See Product Specifications

Related Products

Reagents

Accessories

Cassettes

Instruments

• Specifications

Product Code: MXA020

Orflo Accutase cell detachment solution, 1X, 100 mL

Supporting Resources

Related Products

Reagents

Assays

Antibodies

Cassettes

Instruments

• Specifications

Product Code: MXA021

Orflo Accumax, cell dissassociation reagent, 10X, 100 mL, sterile

Supporting Resources

Related Products

Reagents

Assays

Antibodies

Cassettes

Instruments

• Specifications