Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein.
Many studies have shown that the mycoplasmal membrane protein p37 enhances cancer cell migration, invasion, and metastasis. Previously, we generated 6 monoclonal antibodies (MAbs) against the mycoplasmal protein p37 and showed the presence of mycoplasma-infected circulating tumor cells in the blood...
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doaj-66dc70234d8240f88865d0a36024d0322020-11-24T22:11:27ZengPublic Library of Science (PLoS)PLoS ONE1932-62032016-01-011112e016909110.1371/journal.pone.0169091Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein.Min Kyu KimWon-Tae KimHyun Min LeeHong Seo ChoiYu Ra JoYangsoon LeeJaemin JeongDongho ChoiHee Jin ChangDae Shick KimYoung-Joo JangChun Jeih RyuMany studies have shown that the mycoplasmal membrane protein p37 enhances cancer cell migration, invasion, and metastasis. Previously, we generated 6 monoclonal antibodies (MAbs) against the mycoplasmal protein p37 and showed the presence of mycoplasma-infected circulating tumor cells in the blood of hepatocellular carcinoma patients by using CA27, one of the six MAbs. When mycoplasmas were incubated with cancer cells in the presence of CA27, mycoplasma infection was completely inhibited, suggesting that CA27 is a neutralizing antibody inhibiting mycoplasma infection. To examine the neutralizing epitope of CA27, we generated a series of glutathione S-transferase (GST)-fused p37 deletion mutant proteins in which p37 was partly deleted. To express p37-coding sequences in E.coli, mycoplasmal TGA codons were substituted with TGG in the p37 deletion mutant genes. GST-fused p37 deletion mutant proteins were then screened to identify the epitope targeted by CA27. Western blots showed that CA27 bound to the residues 216-246 on the middle part of the p37 protein while it did not bind to the residues 183-219 and 216-240. Fine mapping showed that CA27 was able to bind to the residues 226-246, but its binding activity was relatively weakened as compared to that to the residues 216-246, suggesting that the residues 226-246 is essential for optimal binding activity of CA27. Interestingly, the treatment of the purified GST-tagged epitopes with urea showed that CA27 binding to the epitope was sodium dodecyl sulfate-resistant but urea-sensitive. The same 226-246 residues were also recognized by two other anti-p37 MAbs, suggesting that the epitope is immunodominant. The identification of the novel neutralizing epitope may provide new insight into the interaction between the p37 protein and host receptors.http://europepmc.org/articles/PMC5201277?pdf=render |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Min Kyu Kim Won-Tae Kim Hyun Min Lee Hong Seo Choi Yu Ra Jo Yangsoon Lee Jaemin Jeong Dongho Choi Hee Jin Chang Dae Shick Kim Young-Joo Jang Chun Jeih Ryu |
spellingShingle |
Min Kyu Kim Won-Tae Kim Hyun Min Lee Hong Seo Choi Yu Ra Jo Yangsoon Lee Jaemin Jeong Dongho Choi Hee Jin Chang Dae Shick Kim Young-Joo Jang Chun Jeih Ryu Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein. PLoS ONE |
author_facet |
Min Kyu Kim Won-Tae Kim Hyun Min Lee Hong Seo Choi Yu Ra Jo Yangsoon Lee Jaemin Jeong Dongho Choi Hee Jin Chang Dae Shick Kim Young-Joo Jang Chun Jeih Ryu |
author_sort |
Min Kyu Kim |
title |
Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein. |
title_short |
Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein. |
title_full |
Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein. |
title_fullStr |
Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein. |
title_full_unstemmed |
Mapping of a Mycoplasma-Neutralizing Epitope on the Mycoplasmal p37 Protein. |
title_sort |
mapping of a mycoplasma-neutralizing epitope on the mycoplasmal p37 protein. |
publisher |
Public Library of Science (PLoS) |
series |
PLoS ONE |
issn |
1932-6203 |
publishDate |
2016-01-01 |
description |
Many studies have shown that the mycoplasmal membrane protein p37 enhances cancer cell migration, invasion, and metastasis. Previously, we generated 6 monoclonal antibodies (MAbs) against the mycoplasmal protein p37 and showed the presence of mycoplasma-infected circulating tumor cells in the blood of hepatocellular carcinoma patients by using CA27, one of the six MAbs. When mycoplasmas were incubated with cancer cells in the presence of CA27, mycoplasma infection was completely inhibited, suggesting that CA27 is a neutralizing antibody inhibiting mycoplasma infection. To examine the neutralizing epitope of CA27, we generated a series of glutathione S-transferase (GST)-fused p37 deletion mutant proteins in which p37 was partly deleted. To express p37-coding sequences in E.coli, mycoplasmal TGA codons were substituted with TGG in the p37 deletion mutant genes. GST-fused p37 deletion mutant proteins were then screened to identify the epitope targeted by CA27. Western blots showed that CA27 bound to the residues 216-246 on the middle part of the p37 protein while it did not bind to the residues 183-219 and 216-240. Fine mapping showed that CA27 was able to bind to the residues 226-246, but its binding activity was relatively weakened as compared to that to the residues 216-246, suggesting that the residues 226-246 is essential for optimal binding activity of CA27. Interestingly, the treatment of the purified GST-tagged epitopes with urea showed that CA27 binding to the epitope was sodium dodecyl sulfate-resistant but urea-sensitive. The same 226-246 residues were also recognized by two other anti-p37 MAbs, suggesting that the epitope is immunodominant. The identification of the novel neutralizing epitope may provide new insight into the interaction between the p37 protein and host receptors. |
url |
http://europepmc.org/articles/PMC5201277?pdf=render |
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