HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell Contact
HIV reactivation from latency is induced by cytokines but also by cell contact with other cells. To better understand this, J1.1 cells, a latent HIV-1-infected Jurkat derivative, were cocultured with its parental Jurkat. J1.1 cells became p17MA-positive and produced a high level of HIV p24CA antigen...
| Published in: | Viruses |
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| Main Authors: | , , , , |
| Format: | Article |
| Language: | English |
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MDPI AG
2020-04-01
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| Online Access: | https://www.mdpi.com/1999-4915/12/4/417 |
| _version_ | 1850412027617476608 |
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| author | Toshiki Okutomi Satoko Minakawa Riku Hirota Koko Katagiri Yuko Morikawa |
| author_facet | Toshiki Okutomi Satoko Minakawa Riku Hirota Koko Katagiri Yuko Morikawa |
| author_sort | Toshiki Okutomi |
| collection | DOAJ |
| container_title | Viruses |
| description | HIV reactivation from latency is induced by cytokines but also by cell contact with other cells. To better understand this, J1.1 cells, a latent HIV-1-infected Jurkat derivative, were cocultured with its parental Jurkat. J1.1 cells became p17MA-positive and produced a high level of HIV p24CA antigen, only when they were cocultured with stimulated Jurkat with cell-to-cell contact. In contrast, very little p24CA was produced when they were cocultured without cell contact. Similar results were obtained when latent ACH-2 and its parental A3.01 cells were cocultured. Confocal microscopy revealed that not only HIV-1 p17MA and gp120Env but also LFA-1, CD81, CD59, and TCR CD3 accumulated at the cell contact site, suggesting formation of the virological synapse-like structure. LFA-1–ICAM-1 interaction was involved in the cell-to-cell contact. When J1.1 was cocultured with TCR-deficient Jurkat, the p17MA-positive rate was significantly lower, although the cell-to-cell contact was not impaired. Quantitative proteomics identified 54 membrane molecules, one of which was MHC class I, that accumulated at the cell contact site. Reactivation from latency was also influenced by the presence of stromal cells. Our study indicated that latent HIV-1 in J1.1/ACH-2 cells was efficiently reactivated by cell-to-cell contact with stimulated parental cells, accompanying the virological synapse-like structure. |
| format | Article |
| id | doaj-art-4bce99eacb704b0c8a5c6a64c3b4c913 |
| institution | Directory of Open Access Journals |
| issn | 1999-4915 |
| language | English |
| publishDate | 2020-04-01 |
| publisher | MDPI AG |
| record_format | Article |
| spelling | doaj-art-4bce99eacb704b0c8a5c6a64c3b4c9132025-08-19T22:46:24ZengMDPI AGViruses1999-49152020-04-0112441710.3390/v12040417HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell ContactToshiki Okutomi0Satoko Minakawa1Riku Hirota2Koko Katagiri3Yuko Morikawa4Graduate School of Infection Control Sciences, Kitasato University, Shirokane 5-9-1, Minato-ku, Tokyo 108-8641, JapanGraduate School of Infection Control Sciences, Kitasato University, Shirokane 5-9-1, Minato-ku, Tokyo 108-8641, JapanGraduate School of Infection Control Sciences, Kitasato University, Shirokane 5-9-1, Minato-ku, Tokyo 108-8641, JapanDepartment of Biosciences, School of Science, Kitasato University, Kitasato 1-15-1, Minami-ku, Sagamihara, Kanagawa 252-0373, JapanGraduate School of Infection Control Sciences, Kitasato University, Shirokane 5-9-1, Minato-ku, Tokyo 108-8641, JapanHIV reactivation from latency is induced by cytokines but also by cell contact with other cells. To better understand this, J1.1 cells, a latent HIV-1-infected Jurkat derivative, were cocultured with its parental Jurkat. J1.1 cells became p17MA-positive and produced a high level of HIV p24CA antigen, only when they were cocultured with stimulated Jurkat with cell-to-cell contact. In contrast, very little p24CA was produced when they were cocultured without cell contact. Similar results were obtained when latent ACH-2 and its parental A3.01 cells were cocultured. Confocal microscopy revealed that not only HIV-1 p17MA and gp120Env but also LFA-1, CD81, CD59, and TCR CD3 accumulated at the cell contact site, suggesting formation of the virological synapse-like structure. LFA-1–ICAM-1 interaction was involved in the cell-to-cell contact. When J1.1 was cocultured with TCR-deficient Jurkat, the p17MA-positive rate was significantly lower, although the cell-to-cell contact was not impaired. Quantitative proteomics identified 54 membrane molecules, one of which was MHC class I, that accumulated at the cell contact site. Reactivation from latency was also influenced by the presence of stromal cells. Our study indicated that latent HIV-1 in J1.1/ACH-2 cells was efficiently reactivated by cell-to-cell contact with stimulated parental cells, accompanying the virological synapse-like structure.https://www.mdpi.com/1999-4915/12/4/417HIV-1latencyreactivationcell-to-cell contactvirological synapse |
| spellingShingle | Toshiki Okutomi Satoko Minakawa Riku Hirota Koko Katagiri Yuko Morikawa HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell Contact HIV-1 latency reactivation cell-to-cell contact virological synapse |
| title | HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell Contact |
| title_full | HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell Contact |
| title_fullStr | HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell Contact |
| title_full_unstemmed | HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell Contact |
| title_short | HIV Reactivation in Latently Infected Cells with Virological Synapse-Like Cell Contact |
| title_sort | hiv reactivation in latently infected cells with virological synapse like cell contact |
| topic | HIV-1 latency reactivation cell-to-cell contact virological synapse |
| url | https://www.mdpi.com/1999-4915/12/4/417 |
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