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Characterization of the Novel CCR5 Lysine
  to Arginine Mutation Using U937 Cells
       A. Clarke, A. Lilly, K. Jones, S.
       Mares, B. Long, A Calvitti, E.
                McCallister
The Family                               IB gave birth to all of her
                                            children naturally, with no
                                            anti-retrovirals.




IIB, the focus of our
research, was exposed
but not infected with
HIV.




  Figure 1. A pedigree showing HIV infection in an African American family.
HIV Isolate Similarity

    HIV isolates from infected family
    members were taken and compared to
    confirm the mother, IB, as the source of
    infection.




Figure 2: Using MacVector, a comparison of genetic distance within the family was modeled.
Child IIB                                                  CCR5 is a gene that codes for a cell
                                                           receptor whose secondary function is
                                                           to act as an HIV co-receptor
                                                           alongside primary receptor CD4.




                                                                                       Location of
                                                                                        Lys to Arg
                                                                                          (TG5)
                                                                                        mutation.




IIB’s CCR5 gene was
sequenced and the lysine to
arginine mutation was
found.


     Figure 3. Amino acid map of the CCR5 receptor showing location of TG5 mutation.
Research Questions/Hypothesis

   What is the function of the TG5 mutated
    gene?
   Does the mutation confer HIV resistance?



   Hypothesis: The CCR5 mutation TG5 does not
        protect a cell from HIV infection.
Overview
To characterize the TG5 mutation, we have decided
upon transfection and transduction techniques to
attempt to express the mutation in U937 promonocytic
human stem cell cancer cells.

U937 cells (pictured in slide backgrounds) were chosen because
the cells possess the CCR5 gene but do not express the
extracellular receptor.
Transfection

                                         The CCR5 allele containing the Lys to Arg
                                         missense mutation observed in subject IIB
                                         was cloned into pcDNA3.1 (Invitrogen).

                                         The map was confirmed by restriction
                                         endonuclease digestion and analysis.

                                         U937 cells were grown in RPMI with 10%
                                         FBS and 1% Pen-Strep (Invitrogen).

                                         Using Lipofectamine 2000
                                         (Invitrogen), U937 cells were transfected
                                         with pcDNATG5.



    Figure 4. Map of constructed transfection plasmid vector pcDNATG5.
Transfection                                          A drug study was done to find the
                                                       optimal amount of G418 to use in
                                                       selection.

                                                       Cells were treated with increasing
                                                       amounts of G418, from 0μg/μL to
                                                       1000μg/μL for a week and counted
                                                       three times.

                                                       Before counting, cells were treated with
                                                       Trypan Blue Stain (Gibco) and dead
                                                       cells took in dye.

                                                       After cells were transfected they were
                                                       treated with 200μg/μL for five weeks.

                                                       Ultimately it the transfection was
                                                       determined to be unsuccessful.


Figure 5. Graph of G418 drug study U937 cell counts.
After transfection proved to be unsuccessful,
Transduction   a transduction using pLNCX2 (Clontech)
               retroviral vector was started.

               First, the vector had to be constructed by
               cutting TG5 out of pcDNA with the use of
               restriction enzymes XbaI and BamHI.

               Oligonucleotide ‘linkers’ were ligated onto
               TG5 which converted the BamHI end into a
               HindIII site, and the XbaI end into a NotI
               site.

               This conversion made TG5 compatible for
               ligation into the Multiple Cloning Site
               (MCS) of pLNCX2.



                                   Figures 6&7. Map of
                                   original pLNCX2
                                   retroviral vector and
                                   MCS sequence.
Transduction
               Now strands of pLNCX2 containing the
               TG5 mutation are being transformed using
               competent E.Coli cells to produce sufficient
               amounts of plasmid for transduction.

               Next, plasmid will be transfected into the
               associated packaging cell line PT67 which
               will assemble the virus particles.

               These particles will be introduced into U937
               cultures, and cells will be allowed to grow.

               Then successfully transduced cells will be
               selected for using the same G418 antibiotics
               used in the transfection.



                     Figure 8. Map of pLNCX2 adapted to show
                     CCR5 TG5 gene.
Future Plans
If the TG5 mutation can be characterized successfully, HIV
infectability may be tested using viral envelope or further testing
if necessary.

We also plan to test any effects of the TG5 mutated gene on both
the CCR5 and CXCR4 (another HIV co-receptor secondary to CD4) receptors.

Provided the mutation is characterized successfully, we will find
another facility to send our cells to in order to test infectability
with actual HIV.

If it is found that the lysine to arginine (TG5) mutation confers
resistance, there are many possibilities for gene therapies, other
treatments, or even a cure.
Acknowledgements
Harry Kestler PhD, Rosa Hainaj PhD, John Crooks
PhD, Margaret Gorensek MD, X. Z. Ma MD, Jalpa
Nagisetty, Jessica Jenkins, Anthony George, Katelyn
Witte, Diana Shuman, Kelly Harrison, and Support of
the Lorain County Community College Foundation


Picture Credits
CCR5 map slide - Figure 3:
www.microbytes.com/blog/2010/07/
pLNCX2 map and MCS - Figure 6&7:
http://www.clontech.com/US/Products/Viral_Transduction/Retroviral_Vector_Systems/C
onstitutive_Promoter?sitex=10020:22372:US

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Characterization of the Novel CCR5 Lysine to Arginine Using U937 Cells

  • 1. Characterization of the Novel CCR5 Lysine to Arginine Mutation Using U937 Cells A. Clarke, A. Lilly, K. Jones, S. Mares, B. Long, A Calvitti, E. McCallister
  • 2. The Family IB gave birth to all of her children naturally, with no anti-retrovirals. IIB, the focus of our research, was exposed but not infected with HIV. Figure 1. A pedigree showing HIV infection in an African American family.
  • 3. HIV Isolate Similarity HIV isolates from infected family members were taken and compared to confirm the mother, IB, as the source of infection. Figure 2: Using MacVector, a comparison of genetic distance within the family was modeled.
  • 4. Child IIB CCR5 is a gene that codes for a cell receptor whose secondary function is to act as an HIV co-receptor alongside primary receptor CD4. Location of Lys to Arg (TG5) mutation. IIB’s CCR5 gene was sequenced and the lysine to arginine mutation was found. Figure 3. Amino acid map of the CCR5 receptor showing location of TG5 mutation.
  • 5. Research Questions/Hypothesis What is the function of the TG5 mutated gene? Does the mutation confer HIV resistance? Hypothesis: The CCR5 mutation TG5 does not protect a cell from HIV infection.
  • 6. Overview To characterize the TG5 mutation, we have decided upon transfection and transduction techniques to attempt to express the mutation in U937 promonocytic human stem cell cancer cells. U937 cells (pictured in slide backgrounds) were chosen because the cells possess the CCR5 gene but do not express the extracellular receptor.
  • 7. Transfection The CCR5 allele containing the Lys to Arg missense mutation observed in subject IIB was cloned into pcDNA3.1 (Invitrogen). The map was confirmed by restriction endonuclease digestion and analysis. U937 cells were grown in RPMI with 10% FBS and 1% Pen-Strep (Invitrogen). Using Lipofectamine 2000 (Invitrogen), U937 cells were transfected with pcDNATG5. Figure 4. Map of constructed transfection plasmid vector pcDNATG5.
  • 8. Transfection A drug study was done to find the optimal amount of G418 to use in selection. Cells were treated with increasing amounts of G418, from 0μg/μL to 1000μg/μL for a week and counted three times. Before counting, cells were treated with Trypan Blue Stain (Gibco) and dead cells took in dye. After cells were transfected they were treated with 200μg/μL for five weeks. Ultimately it the transfection was determined to be unsuccessful. Figure 5. Graph of G418 drug study U937 cell counts.
  • 9. After transfection proved to be unsuccessful, Transduction a transduction using pLNCX2 (Clontech) retroviral vector was started. First, the vector had to be constructed by cutting TG5 out of pcDNA with the use of restriction enzymes XbaI and BamHI. Oligonucleotide ‘linkers’ were ligated onto TG5 which converted the BamHI end into a HindIII site, and the XbaI end into a NotI site. This conversion made TG5 compatible for ligation into the Multiple Cloning Site (MCS) of pLNCX2. Figures 6&7. Map of original pLNCX2 retroviral vector and MCS sequence.
  • 10. Transduction Now strands of pLNCX2 containing the TG5 mutation are being transformed using competent E.Coli cells to produce sufficient amounts of plasmid for transduction. Next, plasmid will be transfected into the associated packaging cell line PT67 which will assemble the virus particles. These particles will be introduced into U937 cultures, and cells will be allowed to grow. Then successfully transduced cells will be selected for using the same G418 antibiotics used in the transfection. Figure 8. Map of pLNCX2 adapted to show CCR5 TG5 gene.
  • 11. Future Plans If the TG5 mutation can be characterized successfully, HIV infectability may be tested using viral envelope or further testing if necessary. We also plan to test any effects of the TG5 mutated gene on both the CCR5 and CXCR4 (another HIV co-receptor secondary to CD4) receptors. Provided the mutation is characterized successfully, we will find another facility to send our cells to in order to test infectability with actual HIV. If it is found that the lysine to arginine (TG5) mutation confers resistance, there are many possibilities for gene therapies, other treatments, or even a cure.
  • 12. Acknowledgements Harry Kestler PhD, Rosa Hainaj PhD, John Crooks PhD, Margaret Gorensek MD, X. Z. Ma MD, Jalpa Nagisetty, Jessica Jenkins, Anthony George, Katelyn Witte, Diana Shuman, Kelly Harrison, and Support of the Lorain County Community College Foundation Picture Credits CCR5 map slide - Figure 3: www.microbytes.com/blog/2010/07/ pLNCX2 map and MCS - Figure 6&7: http://www.clontech.com/US/Products/Viral_Transduction/Retroviral_Vector_Systems/C onstitutive_Promoter?sitex=10020:22372:US