Technique of cultivating limbal derived corneal epithelium on human amniotic membrane for clinical transplantation
Background : The technique of transplantation of cultivated limbal epithelium rather than direct limbal tissue isa novel method of "cell therapy" involved in reconstructing the ocular surface in severe limbal stem celldeficiency [LSCD], caused by chemical burns. Aim : To describe a simple...
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| Veröffentlicht in: | Journal of postgraduate medicine (Bombay) 2006-10, Vol.52 (4), p.257-261 |
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| creator | Fatima A, Sangwan VS, Iftekhar G, Reddy P, Matalia H, Balasubramanian D, Vemuganti GK |
| description | Background : The technique of transplantation of cultivated limbal
epithelium rather than direct limbal tissue isa novel method of "cell
therapy" involved in reconstructing the ocular surface in severe limbal
stem celldeficiency [LSCD], caused by chemical burns. Aim : To describe
a simple feeder-cell free technique of cultivating limbal epithelium on
human amniotic membrane[HAM]. Materials and Methods : The limbal
tissues (2 mm) were harvested from patients with LSCD. These
tissueswere proliferated in vitro on HAM supplemented by human corneal
epithelial cell medium and autologousserum. Cultures covering more
≥50% area of 2.5x5 cm HAM were considered adequate for clinical
use. Thecultured epithelium was characterized by histopathology and
immunophenotyping.Results: A total of 542 cultures out of 250 limbal
tissues were cultivated in the laboratory from January 2001through July
2005. The culture explants showed that clusters of cells emerging from
the edge of the explantsin one-three days formed a complete monolayer
within 10-14 days. In 86% of cultures (464 of 542), thegrowth was
observed within one-two days. Successful explant cultures were observed
in 98.5% (534 of 542cultures) with 91% explant cultures showing an area
of ≥6.25 cm2 (6.25 - 12.5 cm2 range). The cultivatedepithelium
was terminated between 10-14 days for clinical transplantation. The
problems encountered wereinadequate growth (2 of 542) and contamination
(2 of 542). Conclusions : We demonstrate a simple technique of
generating a sheet of corneal epithelium from a limbalbiopsy. This new
technique could pave the way for a novel form of cell therapy. |
| format | Article |
| fullrecord | <record><control><sourceid>gale_proqu</sourceid><recordid>TN_cdi_proquest_miscellaneous_68145716</recordid><sourceformat>XML</sourceformat><sourcesystem>PC</sourcesystem><galeid>A154671805</galeid><sourcerecordid>A154671805</sourcerecordid><originalsourceid>FETCH-LOGICAL-b380t-8a003012d218419984222a6ea74bf81846c54ff9a474ba2be9028c49566ab1e63</originalsourceid><addsrcrecordid>eNptkV1rFTEQhhex2Fr9CxIUereS700uS1ErFLxpr5dsdvacOeRjze4W_Pfm0FZRDglk8vLMyzvMq-aC2o633HDxutaU81YYZc-bt8tyoJRpLcWb5px1jHIl-UVT7sHvE_7cgOSJ-C2s-OhWTDsSMA4ukBEKPsJIfC4J6h9mXPcQcIskJ7LfokvExYR5RU8ixKG4BGTKhfiACX1tWau0zMGltTrn9K45m1xY4P3ze9k8fP1yf3Pb3v349v3m-q4dhKFraxylgjI-cmYks9ZIzrnT4Do5TKZq2is5TdbJKjg-gKXceGmV1m5goMVlc_XkO5dc51vWPuLiIdQgkLel14ZJ1bEj-PE_8JC3kmq2ngtltaDqCH16gnYuQI9pynUsf3Tsr5mSumOGqkq1J6gdJCgu5AQTVvkf_vMJvp4RIvqTDR-es25DhLGfC0ZXfvUvG_3rOGCuC4A_hC_o-hfxMNdLNbVU_Ab9na1M</addsrcrecordid><sourcetype>Aggregation Database</sourcetype><iscdi>true</iscdi><recordtype>article</recordtype><pqid>235963056</pqid></control><display><type>article</type><title>Technique of cultivating limbal derived corneal epithelium on human amniotic membrane for clinical transplantation</title><source>MEDLINE</source><source>Bioline International</source><source>Elektronische Zeitschriftenbibliothek - Frei zugängliche E-Journals</source><creator>Fatima A, Sangwan VS, Iftekhar G, Reddy P, Matalia H, Balasubramanian D, Vemuganti GK</creator><creatorcontrib>Fatima A, Sangwan VS, Iftekhar G, Reddy P, Matalia H, Balasubramanian D, Vemuganti GK</creatorcontrib><description>Background : The technique of transplantation of cultivated limbal
epithelium rather than direct limbal tissue isa novel method of "cell
therapy" involved in reconstructing the ocular surface in severe limbal
stem celldeficiency [LSCD], caused by chemical burns. Aim : To describe
a simple feeder-cell free technique of cultivating limbal epithelium on
human amniotic membrane[HAM]. Materials and Methods : The limbal
tissues (2 mm) were harvested from patients with LSCD. These
tissueswere proliferated in vitro on HAM supplemented by human corneal
epithelial cell medium and autologousserum. Cultures covering more
≥50% area of 2.5x5 cm HAM were considered adequate for clinical
use. Thecultured epithelium was characterized by histopathology and
immunophenotyping.Results: A total of 542 cultures out of 250 limbal
tissues were cultivated in the laboratory from January 2001through July
2005. The culture explants showed that clusters of cells emerging from
the edge of the explantsin one-three days formed a complete monolayer
within 10-14 days. In 86% of cultures (464 of 542), thegrowth was
observed within one-two days. Successful explant cultures were observed
in 98.5% (534 of 542cultures) with 91% explant cultures showing an area
of ≥6.25 cm2 (6.25 - 12.5 cm2 range). The cultivatedepithelium
was terminated between 10-14 days for clinical transplantation. The
problems encountered wereinadequate growth (2 of 542) and contamination
(2 of 542). Conclusions : We demonstrate a simple technique of
generating a sheet of corneal epithelium from a limbalbiopsy. This new
technique could pave the way for a novel form of cell therapy.</description><identifier>ISSN: 0022-3859</identifier><identifier>EISSN: 0972-2823</identifier><identifier>PMID: 17102542</identifier><language>eng</language><publisher>India: Medknow Publications and Staff Society of Seth GS Medical College and KEM Hospital, Mumbai, India</publisher><subject>Amnion ; Amniotic sac ; Cellular therapy ; Corneal epithelium, limbus corneae, stem cell transplantation ; Epithelium, Corneal - growth & development ; Epithelium, Corneal - transplantation ; Eye ; Humans ; Limbus Corneae ; Methods ; Surgery ; Tissue culture ; Tissue Culture Techniques - methods</subject><ispartof>Journal of postgraduate medicine (Bombay), 2006-10, Vol.52 (4), p.257-261</ispartof><rights>Copyright 2006 Journal of Postgraduate Medicine.</rights><rights>COPYRIGHT 2006 Medknow Publications and Media Pvt. Ltd.</rights><rights>Copyright Medknow Publications Oct-Dec 2006</rights><lds50>peer_reviewed</lds50><oa>free_for_read</oa><woscitedreferencessubscribed>false</woscitedreferencessubscribed></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Tsyndetics_thumb_exl</thumbnail><link.rule.ids>314,776,780,79168</link.rule.ids><backlink>$$Uhttps://www.ncbi.nlm.nih.gov/pubmed/17102542$$D View this record in MEDLINE/PubMed$$Hfree_for_read</backlink></links><search><creatorcontrib>Fatima A, Sangwan VS, Iftekhar G, Reddy P, Matalia H, Balasubramanian D, Vemuganti GK</creatorcontrib><title>Technique of cultivating limbal derived corneal epithelium on human amniotic membrane for clinical transplantation</title><title>Journal of postgraduate medicine (Bombay)</title><addtitle>J Postgrad Med</addtitle><description>Background : The technique of transplantation of cultivated limbal
epithelium rather than direct limbal tissue isa novel method of "cell
therapy" involved in reconstructing the ocular surface in severe limbal
stem celldeficiency [LSCD], caused by chemical burns. Aim : To describe
a simple feeder-cell free technique of cultivating limbal epithelium on
human amniotic membrane[HAM]. Materials and Methods : The limbal
tissues (2 mm) were harvested from patients with LSCD. These
tissueswere proliferated in vitro on HAM supplemented by human corneal
epithelial cell medium and autologousserum. Cultures covering more
≥50% area of 2.5x5 cm HAM were considered adequate for clinical
use. Thecultured epithelium was characterized by histopathology and
immunophenotyping.Results: A total of 542 cultures out of 250 limbal
tissues were cultivated in the laboratory from January 2001through July
2005. The culture explants showed that clusters of cells emerging from
the edge of the explantsin one-three days formed a complete monolayer
within 10-14 days. In 86% of cultures (464 of 542), thegrowth was
observed within one-two days. Successful explant cultures were observed
in 98.5% (534 of 542cultures) with 91% explant cultures showing an area
of ≥6.25 cm2 (6.25 - 12.5 cm2 range). The cultivatedepithelium
was terminated between 10-14 days for clinical transplantation. The
problems encountered wereinadequate growth (2 of 542) and contamination
(2 of 542). Conclusions : We demonstrate a simple technique of
generating a sheet of corneal epithelium from a limbalbiopsy. This new
technique could pave the way for a novel form of cell therapy.</description><subject>Amnion</subject><subject>Amniotic sac</subject><subject>Cellular therapy</subject><subject>Corneal epithelium, limbus corneae, stem cell transplantation</subject><subject>Epithelium, Corneal - growth & development</subject><subject>Epithelium, Corneal - transplantation</subject><subject>Eye</subject><subject>Humans</subject><subject>Limbus Corneae</subject><subject>Methods</subject><subject>Surgery</subject><subject>Tissue culture</subject><subject>Tissue Culture Techniques - methods</subject><issn>0022-3859</issn><issn>0972-2823</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2006</creationdate><recordtype>article</recordtype><sourceid>RBI</sourceid><sourceid>EIF</sourceid><sourceid>8G5</sourceid><sourceid>BENPR</sourceid><sourceid>GUQSH</sourceid><sourceid>M2O</sourceid><recordid>eNptkV1rFTEQhhex2Fr9CxIUereS700uS1ErFLxpr5dsdvacOeRjze4W_Pfm0FZRDglk8vLMyzvMq-aC2o633HDxutaU81YYZc-bt8tyoJRpLcWb5px1jHIl-UVT7sHvE_7cgOSJ-C2s-OhWTDsSMA4ukBEKPsJIfC4J6h9mXPcQcIskJ7LfokvExYR5RU8ixKG4BGTKhfiACX1tWau0zMGltTrn9K45m1xY4P3ze9k8fP1yf3Pb3v349v3m-q4dhKFraxylgjI-cmYks9ZIzrnT4Do5TKZq2is5TdbJKjg-gKXceGmV1m5goMVlc_XkO5dc51vWPuLiIdQgkLel14ZJ1bEj-PE_8JC3kmq2ngtltaDqCH16gnYuQI9pynUsf3Tsr5mSumOGqkq1J6gdJCgu5AQTVvkf_vMJvp4RIvqTDR-es25DhLGfC0ZXfvUvG_3rOGCuC4A_hC_o-hfxMNdLNbVU_Ab9na1M</recordid><startdate>20061001</startdate><enddate>20061001</enddate><creator>Fatima A, Sangwan VS, Iftekhar G, Reddy P, Matalia H, Balasubramanian D, Vemuganti GK</creator><general>Medknow Publications and Staff Society of Seth GS Medical College and KEM Hospital, Mumbai, India</general><general>Medknow Publications and Media Pvt. 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epithelium rather than direct limbal tissue isa novel method of "cell
therapy" involved in reconstructing the ocular surface in severe limbal
stem celldeficiency [LSCD], caused by chemical burns. Aim : To describe
a simple feeder-cell free technique of cultivating limbal epithelium on
human amniotic membrane[HAM]. Materials and Methods : The limbal
tissues (2 mm) were harvested from patients with LSCD. These
tissueswere proliferated in vitro on HAM supplemented by human corneal
epithelial cell medium and autologousserum. Cultures covering more
≥50% area of 2.5x5 cm HAM were considered adequate for clinical
use. Thecultured epithelium was characterized by histopathology and
immunophenotyping.Results: A total of 542 cultures out of 250 limbal
tissues were cultivated in the laboratory from January 2001through July
2005. The culture explants showed that clusters of cells emerging from
the edge of the explantsin one-three days formed a complete monolayer
within 10-14 days. In 86% of cultures (464 of 542), thegrowth was
observed within one-two days. Successful explant cultures were observed
in 98.5% (534 of 542cultures) with 91% explant cultures showing an area
of ≥6.25 cm2 (6.25 - 12.5 cm2 range). The cultivatedepithelium
was terminated between 10-14 days for clinical transplantation. The
problems encountered wereinadequate growth (2 of 542) and contamination
(2 of 542). Conclusions : We demonstrate a simple technique of
generating a sheet of corneal epithelium from a limbalbiopsy. This new
technique could pave the way for a novel form of cell therapy.</abstract><cop>India</cop><pub>Medknow Publications and Staff Society of Seth GS Medical College and KEM Hospital, Mumbai, India</pub><pmid>17102542</pmid><tpages>5</tpages><oa>free_for_read</oa></addata></record> |
| fulltext | fulltext |
| identifier | ISSN: 0022-3859 |
| ispartof | Journal of postgraduate medicine (Bombay), 2006-10, Vol.52 (4), p.257-261 |
| issn | 0022-3859 0972-2823 |
| language | eng |
| recordid | cdi_proquest_miscellaneous_68145716 |
| source | MEDLINE; Bioline International; Elektronische Zeitschriftenbibliothek - Frei zugängliche E-Journals |
| subjects | Amnion Amniotic sac Cellular therapy Corneal epithelium, limbus corneae, stem cell transplantation Epithelium, Corneal - growth & development Epithelium, Corneal - transplantation Eye Humans Limbus Corneae Methods Surgery Tissue culture Tissue Culture Techniques - methods |
| title | Technique of cultivating limbal derived corneal epithelium on human amniotic membrane for clinical transplantation |
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