עבודה זו נתמכה על ידי NIH מענק EY 012,031 (ET-A), פרס קרן קירבי FM (ET-A), מחקר למניעה, עיוורון Inc (MAZ), ניו ג&#39;רזי האריות Eye Research Foundation (MAZ), מכון עיניים של ניו ג&#39;רזי (MAZ), את ג&#39;יי ג&#39;וזף מרגריט DiSepio רשתית מחקר קרן (MAZ), ואת מיטשל ג&#39;ניס ואסאר ואשבי מיטשל Fellowship (AMK).

1. ביצוע לעמוד בהזמנה אישית עבור מוסיף תרבית תאים הבסיס של 5 מ&quot;ל פיפטה קצה (ISC BioExpress, # P-3250-19) הוא בעל קוטר פנימי של 13 מ&quot;מ, אשר בהחלט מתאים לגודל התחתון (12.6 מ&quot;מ, קוטרו החיצוני) של 10 מ&quot;מ (קוטר פנימי) תא NUNC הכנס תרבות (8 מיקרומטר, פוליקרבונט הממברנה, תרמי, # 137443). כדי להפוך את העמדה, פיפטה נותק סמוך לבסיס כדי לייצר גליל 6 מ&quot;מ חלול ארוך. ואז, הוסרו חלקים מהצד של גליל באמצעות להב להבה מחוממים כדי ליצור 3 רגליים (4 מ&quot;מ גובה) תחת טבעת (2 מ&quot;מ גובה), אשר העלה את גובה הכנסות על ידי כ 5 מ&quot;מ. 2. הכנת נייר סינון סטרילי עבור התקשרות והתרבות של הרשתית חזירי Whatman 4M נייר סינון (חתול מס &#39;1004) נחתך לצורה עגולה (6.3 מ&quot;מ קוטר) עם ידית, משולש קטן ששימש להעברת הנייר לסנן לתוך שפופרת זכוכית עבור עיקור או פעם הרשתית צורף (כמו המוצג בסרטון). 3. הכנת explants רשתית עיניים מ - 5 חודשים-9 הישן, 150-230 ק&quot;ג, אמריקן חזירים יורקשייר התקבלו שחיטה מקומית בתוך שלוש שעות של enucleation (מועבר על הקרח). עם ההגעה, העיניים נוקו של רקמת זרים, טבול פתרון בבטאדין (10% Povidone-יוד, החברה פרדריק פרדו, סטמפורד, CT) ורחץ פעמיים השתנה Dulbecco הנשר בינוני (DMEM עם גלוקוז 1g / L, L-גלוטמין, ו pyruvate נתרן, Cellgro-mediatech Inc, Manasses, VA) בתוספת 2.5 מיקרוגרם / מ&quot;ל ​​amphotericin B (Gibco-Invitrogen, בקרלסבד, קליפורניה). פלח קדמי הוסר, חשיפת הרשתית העצבית. ששת מ&quot;מ להבים המקדחה (Storz עיניים, באוש לומב, מנצ&#39;סטר, MO) שימשו לחתוך המשוונית, עובי מלא explants קטע האחורי. הרשתית היה קלופים לאחר מכן את ידי בעדינות החלת פיסת נייר יבש מסנן סטרילי על שכבת תא הגנגליון, מרימים את הרשתית העצבית, ומעמידים את הנייר עם מסנן הרשתית מחוברים על להכניס את התרבות, photoreceptors פונה כלפי מעלה. הכנס הושם מכן לתוך בינוני תרבות, והקפד לכסות באופן מלא את הרשתית, בצלחת 12 גם תרבות (פישר). Explants מרובים הושגו שגרתי תרבותי מן העין אחת. 4. רקמות תרבות רקמת הרשתית היה בתרבית בינוני Essential Minimum הנשר (ממ, Invitrogen-Gibco-Life טכנולוגיות בע&quot;מ, Rockville, MD), pH 7.4, בתוספת 0.2 מ&quot;ג / מ&quot;ל ​​גלוטמין, 10 מיקרוגרם / מ&quot;ל ​​אינסולין חזירי, pyruvate 1 מ&quot;מ, 0.1 L-חומצה אסקורבית מ&quot;מ, 100 U / ml פניצילין, 100 מיקרוגרם / מ&quot;ל סטרפטומיצין, ו 250 ng / ml amphotericin B (אנטיביוטי Antimycotic: Sigma, סנט לואיס, מיזורי), ואת סודה עם 5% CO 2 humidified, האוויר איזון, בשעה 37 ° C. בינוני הוחלפה כל יומיים. רקמות יכול לשמש, מטופלים עם מגוון רחב של חומרים כימיים או בדיקות, או מטופל עבור ניתוחים ביוכימיים או מורפולוגיים הבאים. הקטע שלהלן מתאר את הנהלים כדי ליצור עקביות עובי הרשתית מלא חתכים. 5. חתך <ol style=";text-align:right;direction:rtl"><li style=";text-align:right;direction:rtl"> שימוש cryostat <ol style=";text-align:right;direction:rtl"><li style=";text-align:right;direction:rtl"> תיקון רקמת הרשתית ב parafomaldehyde 4% בין לילה ב 4 מעלות צלזיוס; </li><li style=";text-align:right;direction:rtl"> יש לשטוף את רקמת בקצרה עם פוספט שנאגרו מלוחים (PBS); </li><li style=";text-align:right;direction:rtl"> בזהירות להסיר את הרקמה מנייר מסנן בזמן שהוא ב-PBS בצלחת 35 מ&quot;מ באמצעות מיקרוסקופ לנתיחה; </li><li style=";text-align:right;direction:rtl"> העברת רקמות סוכרוז 30% ולשמור לילה ב 4 מעלות צלזיוס; </li><li style=";text-align:right;direction:rtl"> יניקה משם את הפתרון עודף סביב הרקמה, להוסיף מספיק רקמות-Tek בינוני (מתחם אוקטובר 4583) כדי לכסות את הרקמה, ולתת לו להשרות בטמפרטורת החדר למשך 2 שעות לחדור רקמות; </li><li style=";text-align:right;direction:rtl"> בניית מסגרת רבועה (10 מ&quot;מ x 10 מ&quot;מ, גובה 5 מ&quot;מ) עם שעווה שיניים למקם אותו סביב הרקמה; להוסיף יותר רקמות-Tek בינוני כדי למלא את המסגרת (לוודא את דגימת רקמות שטוחה) ומניחים במקפיא (- 20 ° C) לפחות שעה 1; </li><li style=";text-align:right;direction:rtl"> מעבירים את גוש מדגם קפוא פלטפורמה מדגם (לוודא לחסום מדגם אנכי לבמה); </li><li style=";text-align:right;direction:rtl"> הר פלטפורמה מדגם cryostat מראש מקורר (-20 ° C, לייקה, CM1900) ולוודא לחסום הוא אנכי להב; </li><li style=";text-align:right;direction:rtl"> הסרת שעווה לחסום מסגרת לפני חתך את הרקמה על עובי הרצוי; </li><li style=";text-align:right;direction:rtl"> מניחים את הסעיפים על ג&#39;לטין שטופלו שקופיות. </li></ol></li><li style=";text-align:right;direction:rtl"> שימוש Vibratome <ol style=";text-align:right;direction:rtl"><li style=";text-align:right;direction:rtl"> תקן ולשטוף את הרקמה כפי שתואר לעיל עבור cryostat; </li><li style=";text-align:right;direction:rtl"> הנח את רקמת לתוך אגר, מחומם מראש 4% מומס במיכל קטן ולשמור על 4 מעלות צלזיוס עד נקרש אגר לחלוטין; </li><li style=";text-align:right;direction:rtl"> השתמש בלהב חד לחתוך את אגר לגוש קטן עם מדגם רקמות בפנים; </li><li style=";text-align:right;direction:rtl"> ההדבקה מדגם בלוק על בעל מדגם vibratome בדבק מגע עם דבק (לוודא את פיסת רקמה מדגם אנכי לפלטפורמה של הדואר בעל המדגם, כלומר, בניצב להב) ואת הר בעל חתך על מערכת vibratome (לייקה, סדרה 1000) עם לחסום את המדגם שקוע לחלוטין במי קרח; </li><li style=";text-align:right;direction:rtl"> חותכים את גוש מדגם לתוך 50 מיקרומטר חלקים ומניחים אותם על ג&#39;לטין שטופלו שקופיות עם מברשת רכה. </li></ol></li></ol> 6. אימונוהיסטוכימיה השתמש בכל הפרוטוקול הסטנדרטי. חלקים עבים Immunolabeled ניתן לצפות באמצעות מיקרוסקופ confocal. 7. נציג תוצאות: מורפולוגיה השתמרה במשך שבעת הימים של התרבות. תמונות של הרשתית לפני ואחרי culturing זמינים הווידאו.

<ol>
	<li>Johnson, T. V., Martin, K. R. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Development+and+characterization+of+an+adult+retinal+explant+organotypic+tissue+culture+system+as+an+in+vitro+intraocular+stem+cell+transplantation+model.">Development and characterization of an adult retinal explant organotypic tissue culture system as an in vitro intraocular stem cell transplantation model.</a> Invest Ophthalmol Vis Sci. 49, 3503-3512 (2008).</li><li>Kretz, A., Marticke, J. K., Happold, C. J., Schmeer, C., Isenmann, S. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+primary+culture+technique+of+adult+retina+for+regeneration+studies+on+adult+CNS+neurons.">A primary culture technique of adult retina for regeneration studies on adult CNS neurons.</a> Nat Protoc. 2, 131-140 (2007).</li><li>Donovan, S. L., Dyer, M. A. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Preparation+and+square+wave+electroporation+of+retinal+explant+cultures.">Preparation and square wave electroporation of retinal explant cultures.</a> Nat Protoc. 1, 2710-2718 (2006).</li><li>Koizumi, A., Zeck, G., Ben, Y., Masland, R. H., Jakobs, T. C. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Organotypic+culture+of+physiologically+functional+adult+mammalian+retinas.">Organotypic culture of physiologically functional adult mammalian retinas.</a> PLoS One. 2, e221-e221 (2007).</li><li>Lye, M. H., Jakobs, T. C., Masland, R. H., Koizumi, A. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Organotypic+culture+of+adult+rabbit+retina.">Organotypic culture of adult rabbit retina.</a> J Vis Exp. , (2007).</li><li>Ames, A., Li, Y. Y., Heher, E. C., Kimble, C. R. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Energy+metabolism+of+rabbit+retina+as+related+to+function:+high+cost+of+Na++transport.">Energy metabolism of rabbit retina as related to function: high cost of Na+ transport.</a> J Neurosci. 12, 840-853 (1992).</li><li>Kobuch, K. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Maintenance+of+adult+porcine+retina+and+retinal+pigment+epithelium+in+perfusion+culture:+characterisation+of+an+organotypic+in+vitro+model.">Maintenance of adult porcine retina and retinal pigment epithelium in perfusion culture: characterisation of an organotypic in vitro model.</a> Exp Eye Res. 86, 661-668 (2008).</li><li>Kaempf, S., Walter, P., Salz, A. K., Thumann, G. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Novel+organotypic+culture+model+of+adult+mammalian+neurosensory+retina+in+co-culture+with+retinal+pigment+epithelium.">Novel organotypic culture model of adult mammalian neurosensory retina in co-culture with retinal pigment epithelium.</a> J Neurosci Methods. 173, 47-58 (2008).</li><li>Guduric-Fuchs, J. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Immunohistochemical+study+of+pig+retinal+development.">Immunohistochemical study of pig retinal development.</a> Mol Vis. 15, 1915-1928 (2009).</li><li>Chandler, M. J., Smith, P. J., Samuelson, D. A., MacKay, E. O. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Photoreceptor+density+of+the+domestic+pig+retina.">Photoreceptor density of the domestic pig retina.</a> Vet Ophthalmol. 2, 179-184 (1999).</li></ol>

אין ניגודי אינטרסים הכריז.

החוקרים Vision הקימו מגוון רחב של מערכות תרבות ברשתית, כולל מערכות organotypic, ללמוד מגוון רחב של נושאים, כגון תא גזע השתלת רשתית 1, התחדשות הרשתית 2, ביטוי גנים אקסוגניים 3-5. עם זאת, הרשתית יונקים בוגרים קשה לשמור במבחנה, בעיקר בשל אנרגיה גבוהה לדרישות phot...

<table border="1" style=";text-align:right;direction:rtl"><tbody><tr><td> שם מגיב </td><td> חברה </td><td> מספר קטלוגי </td><td> תגובות </td></tr><tr><td> מ </td><td> Invitrogen-Gibco </td><td> 10370-021 </td><td></td></tr><tr><td> 5 מ&quot;ל פיפטה קצה </td><td> ISC BioExpress </td><td> P-3250-19 </td><td></td></tr><tr><td> תרבות NUNC תא להכניס </td><td> תרמי </td><td> 137443 </td><td> 8μm, פוליקרבונט </td></tr><tr><td> Whatman נייר סינון 4M </td><td> Whatman </td><td> 1004 </td><td></td></tr><tr><td> DMEM </td><td> Cellgro-mediatech Inc </td><td> 10-013-CV </td><td></td></tr><tr><td> אגר </td><td> Fluka </td><td> 05040 </td><td></td></tr><tr><td> Fungizone amphotericin B </td><td> Invitrogen-Gibco </td><td> 15290018 </td><td></td></tr><tr><td> המקדחה להבי </td><td> באוש לומב </td><td> T3096 </td><td> 6.00mm </td></tr><tr><td> אוקטובר מתחם </td><td> מיקרוסקופית אלקטרונים למדעים </td><td> 62550-01 </td><td> 4583 </td></tr><tr><td></td><td> למדעים </td><td></td><td></td></tr><tr><td> Cryostat </td><td> לייקה </td><td> CM1900 </td><td></td></tr><tr><td> Vibratome </td><td> לייקה </td><td> סדרה 1000 </td><td></td></tr><tr><td> Confocal מיקרוסקופית; </td><td> Carl Zeiss </td><td> LSM510 </td><td></td></tr><tr><td> Anti-Synaptic שלפוחיות חלבון 2 (SV2) נוגדנים חד שבטיים העכבר </td><td> DSHB </td><td> N / A </td><td></td></tr><tr><td> נגד גליה Fibrillary חומציים חלבון (GFAP) נוגדן ארנבת polyclonal </td><td> DAKO </td><td> DAKO </td><td></td></tr><tr><td> Propidium יודיד (PI) </td><td> סיגמא </td><td> P4170 </td><td></td></tr></tbody></table>

organotypic culture of full-thickness adult porcine retina

יש ביקוש מוכר במודלים חוץ גופית זה יכול להחליף או לצמצם את הניסויים בבעלי חיים. הרשתית חזירי יש מבנה עצבי דומה הרשתית האנושית ולכן הוא זן בעל ערך לחקר המנגנונים של פגיעה ברשתית האנושית מחלה ניוונית. כאן אנו מתארים שיטה חסכונית לתרבות organotypic של הרשתית חזירי מבוגר מבודד מעיני המתקבל מטבחיים. לאחר הסרת פלח קדמי, להב המקדחה נעשה שימוש כדי ליצור מספר רב של עצבי הרשתית, ברוך קרום הרשתית, דמית העין, בלובן העין של explants מן קטע האחורי של העיניים חזירי מבוגר. פיסת נייר סינון סטרילי שימש להרים את הרשתית העצבית מן explant כל אחד. המתחם מסנן נייר הרשתית היה מתורבת (צד photoreceptor ומעלה) על גבי להוסיף, שהתקיים הרחק בתחתית הצלחת לעמוד על ידי תרבות מחוייט. לעמוד מאפשרת זרימת טוב של המדיום תרבות על שני הצדדים של הרשתית. ככלל, הליך זה הוא פשוט, לשחזור, ומאפשרת שימור של מבנה הרשתית יליד לפחות שבעה ימים, מה שהופך אותו מודל שימושי עבור מגוון רחב של מחקרים מורפולוגיים, תרופתי, ו ביוכימי על הרשתית יונקים.

Watch this Scientific Journal Video about Organotypic Culture of Full-thickness Adult Porcine Retina at JoVE.com

Organotypic Culture of Full-thickness Adult Porcine Retina

כאן אנו מתארים שיטה חסכונית לתרבות organotypic של הרשתית חזירי הבוגרת במשך שבעה ימים. בקצרה, נייר סינון סטרילי שימש להרים את הרשתית העצבית מן הרשתית ואת photoreceptor מקום על הצד להוסיף שהעלו לעמוד מחוייט.

תרבות Organotypic של הרשתית מלא עובי למבוגרים חזירי

There is a recognized demand for in vitro models that can replace or reduce animal experiments. Porcine retina has a similar neuronal structure to human ...

organotypic-culture-of-full-thickness-adult-porcine-retina

Research

JoVE Journal

Neuroscience

14.9K Views.  University of Medicine and Dentistry of New Jersey - UMDNJ. כאן אנו מתארים שיטה חסכונית לתרבות organotypic של הרשתית חזירי הבוגרת במשך שבעה ימים. בקצרה, נייר סינון סטרילי שימש להרים את הרשתית העצבית מן הרשתית ואת photoreceptor מקום על הצד להוסיף שהעלו לעמוד מחוייט.

Video: Organotypic Culture of Full-thickness Adult Porcine Retina

The Organotypic Hippocampal Slice Culture Model for Examining Neuronal Injury

Organotypic hippocampal slice culture is an in vitro method to examine mechanisms of neuronal injury in which the basic architecture and composition of the hippocampus is relatively preserved 1. The organotypic culture system allows for the examination of neuronal, astrocytic and microglial effects, but as an ex vivo preparation, does not address effects of blood flow, or recruitment of peripheral inflammatory cells. To that end, this culture method is frequently used to examine excitotoxic and hypoxic injury to pyramidal neurons of the hippocampus, but has also been used to examine the inflammatory response. Herein we describe the methods for generating hippocampal slice cultures from postnatal rodent brain, administering toxic stimuli to induce neuronal injury, and assaying and quantifying hippocampal neuronal death.

The organoptypic hippocampal slice culture model is an in vitro model used to examine neuronal injury in a variety of paradigms. In this article, we describe the methods for generating slice cultures and quantifying neuronal injury.

תרבות Organotypic בהיפוקמפוס Slice דגם לבחינת פגיעה עצבית

Organotypic hippocampal slice culture is an in vitro method to examine mechanisms of neuronal injury in which the basic architecture and composition of ...

Organotypic Slice Culture of GFP-expressing Mouse Embryos for Real-time Imaging of Peripheral Nerve Outgrowth

For many purposes, the cultivation of mouse embryos ex vivo as organotypic slices is desirable. For example, we employ a transgenic mouse line (tauGFP) in which the enhanced version of the green fluorescent protein (EGFP) is exclusively expressed in all neurons of the developing central and peripheral nervous system1, allowing the possibility to both film the innervation of the forelimb and to manipulate this process with pharmacological and genetic techniques2. The most critical parameter in the successful cultivation of such slice cultures is the method by which the slices are prepared. After extensive testing of a variety of methods, we have found that a vibratome is the best possible device to slice the embryos such that they routinely result in a culture that demonstrates viability over a period of several days, and most importantly, develops in an age-specific manner. For mid-gestation embryos, this includes the normal outgrowth of spinal nerves from the spinal cord and the dorsal root ganglia to their targets in the periphery and the proper determination of skeletal and muscle tissue. 
In this work, we present a method for processing whole embryos of embryonic day (E) E10 to E12 into 300 - 400 micrometer slices for cultivation in a standard tissue culture incubator, which can be studied for up to two days after slice preparation. Critical for the success of this approach is the use of a vibratome to slice each agarose-embedded embryo. This is followed by the cultivation of the slices upon Millicell culture membrane inserts placed upon a small volume of medium, resulting in an interface culture technique. One litter with an average of 7 embryos routinely produces at least 14 slices (2-3 slices of the forelimb region per embryo), which varies slightly due to the age of the embryos as well as to the thickness of the slices. About 80% of the cultured slices show nerve outgrowth, which can be measured througout the culturing period2. Representative results using the tauGFP mouse line are demonstrated.

We present a method to prepare organotypic slices of mid-gestation mouse embryos for the cultivation and time-lapse imaging of peripheral nerve outgrowth.

פורסים תרבות Organotypic של ה-GFP-לבטא עוברי עכברים עבור הדמיה בזמן אמת תולדה של עצבים היקפיים

For many purposes, the cultivation of mouse embryos ex vivo as organotypic slices is desirable. For example, we employ a transgenic mouse line (tauGFP) in ...

In vivo Electroporation of Developing Mouse Retina

The functional characterization of genes expressed during mammalian retinal development remains a significant challenge. Gene targeting to generate constitutive or conditional loss of function knockouts remains cost and labor intensive, as well as time consuming. Adding to these challenges, retina expressed genes may have essential roles outside the retina leading to unintended confounds when using a knockout approach. Furthermore, the ability to ectopically express a gene in a gain of function experiment can be extremely valuable when attempting to identify a role in cell fate specification and/or terminal differentiation.
We present a method for the rapid and efficient incorporation of DNA plasmids into the neonatal mouse retina by electroporation. The application of short electrical impulses above a certain field strength results in a transient increase in plasma membrane permeability, facilitating the transfer of material across the membrane 1,2,3,4. Groundbreaking work demonstrated that electroporation could be utilized as a method of gene transfer into mammalian cells by inducing the formation of hydrophilic plasma membrane pores allowing the passage of highly charged DNA through the lipid bilayer 5. Continuous technical development has resulted in the viability of electroporation as a method for in vivo gene transfer in multiple mouse tissues including the retina, the method for which is described herein 6, 7, 8, 9, 10. 
DNA solution is injected into the subretinal space so that DNA is placed between the retinal pigmented epithelium and retina of the neonatal (P0) mouse and electrical pulses are applied using a tweezer electrode. The lateral placement of the eyes in the mouse allows for the easy orientation of the tweezer electrode to the necessary negative pole-DNA-retina-positive pole alignment. Extensive incorporation and expression of transferred genes can be identified by postnatal day 2 (P2). Due to the lack of significant lateral migration of cells in the retina, electroporated and non-electroporated regions are generated. Non-electroporated regions may serve as internal histological controls where appropriate. 
Retinal electroporation can be used to express a gene under a ubiquitous promoter, such as CAG, or to disrupt gene function using shRNA constructs or Cre-recombinase. More targeted expression can be achieved by designing constructs with cell specific gene promoters. Visualization of electroporated cells is achieved using bicistronic constructs expressing GFP or by co-electroporating a GFP expression construct. Furthermore, multiple constructs may be electroporated for the study of combinatorial gene effects or simultaneous gain and loss of function of different genes. Retinal electroporation may also be utilized for the analysis of genomic cis-regulatory elements by generating appropriate expression constructs and deletion mutants. Such experiments can be used to identify cis-regulatory regions sufficient or required for cell specific gene expression 11. Potential experiments are limited only by construct availability.

In vivo Electroporation of Developing Mouse Retina

A method for the incorporation of plasmid DNA into murine retinal cells for the purpose of performing either gain- or loss of function studies in vivo is presented. This method capitalizes on the transient increase in permeability of cell plasma membranes induced by the application of an external electrical field.

ב electroporation vivo של הרשתית עכבר פיתוח

The functional characterization of genes expressed during mammalian retinal development remains a significant challenge.  Gene targeting to generate ...

Isolation and Culture of Adult Neural Stem Cells from the Mouse Subcallosal Zone

Adult neural stem cells (aNSCs) can be used for the regeneration of damaged brain tissue. NSCs have the potential for differentiation and proliferation into three types of cells: neurons, astrocytes, and oligodendrocytes. Identifying aNSC-derived regions and characterizing the aNSC properties are critical for the potential use of aNSCs and for the elucidation of their role in neural regeneration. The subcallosal zone (SCZ), located between white matter and the hippocampus, has recently been reported to contain aNSCs and continuously give rise to neuroblasts. A low percentage of aNSCs from the SCZ is differentiated into neurons; most cells are differentiated into glial cells, such as oligodendrocytes and astrocytes. These cells are suggested to have a therapeutic potential for traumatic cortical injury. This protocol describes in detail the process to generate SCZ-aNSCs from an adult mouse brain. A brain matrix with intervals of 1 mm is used to obtain the SCZ-containing coronal slices and to precisely dissect the SCZ from the whole brain. The SCZ sections are initially subjected to a neurosphere culture. A well-developed culture system allows for the verification of their characteristics and can increase research on NSCs. A neurosphere culture system provides a useful tool for determining proliferation and collecting the genuine NSCs. A monolayer culture is also an in vitro system to assay proliferation and differentiation. Significantly, this culture system provides a more homogenous environment for NSCs than the neurosphere culture system. Thus, using a discrete brain region, these culture systems will be helpful for expanding our knowledge about aNSCs and their applications for therapeutic uses.

Establishing culture systems for the expansion of adult neural stem cells (aNSCs) allows for the examination and application of aNSCs for therapy. The subcallosal zone (SCZ) has recently been recognized as a novel neuroblast-forming region in adult mice. Here, methods for the isolation, expansion, and differentiation of SCZ-aNSCs are described.

בידוד והתרבות של תאי גזע בוגרים עצביים מאזור העכבר Subcallosal

Adult neural stem cells (aNSCs) can be used for the regeneration of damaged brain tissue. NSCs have the potential for differentiation and proliferation ...

Preparation of Horizontal Slices of Adult Mouse Retina for Electrophysiological Studies

Vertical slice preparations are well established to study circuitry and signal transmission in the adult mammalian retina. The plane of sectioning in these preparations is perpendicular to the retinal surface, making it ideal for the study of radially oriented neurons like photoreceptors and bipolar cells. However, the large dendritic arbors of horizontal cells, wide-field amacrine cells, and ganglion cells are mostly truncated, leaving markedly reduced synaptic activity in these cells. Whereas ganglion cells and displaced amacrine cells can be studied in a whole-mounted preparation of the retina, horizontal cells and amacrine cells located in the inner nuclear layer are only poorly accessible for electrodes in whole retina tissue.
To achieve maximum accessibility and synaptic integrity, we developed a horizontal slice preparation of the mouse retina, and studied signal transmission at the synapse between photoreceptors and horizontal cells. Horizontal sectioning allows&#160;(1) easy and unambiguous visual identification of horizontal cell bodies for electrode targeting, and (2) preservation of the extended horizontal cell dendritic fields, as a prerequisite for intact and functional cone synaptic input to horizontal cell dendrites.
Horizontal cells from horizontal slices exhibited tonic synaptic activity in the dark, and they responded to brief flashes of light with a reduction of inward current and diminished synaptic activity. Immunocytochemical evidence indicates that almost all cones within the dendritic field of a horizontal cell establish synapses with its peripheral dendrites. The horizontal slice preparation is therefore well suited to study the physiological properties of horizontally extended retinal neurons as well as sensory signal transmission and integration across selected synapses.

We developed a horizontal slice preparation of the adult mammalian retina with the plane of sectioning parallel to the retinal surface. Dendritic fields of nonradially oriented retinal neurons were not truncated, allowing the study of signal processing with patch-clamp and imaging techniques.

הכנת פרוסות אופקיות של רשתית למבוגרים עכבר עבור אלקטרו מחקרים

Vertical slice preparations are well established to study circuitry and signal transmission in the adult mammalian retina. The plane of sectioning in ...

Time-lapse Confocal Imaging of Migrating Neurons in Organotypic Slice Culture of Embryonic Mouse Brain Using In Utero Electroporation

In utero electroporation is a rapid and powerful approach to study the process of radial migration in the cerebral cortex of developing mouse embryos. It has helped to describe the different steps of radial migration and characterize the molecular mechanisms controlling this process. To directly and dynamically analyze migrating neurons they have to be traced over time. This protocol describes a workflow that combines in utero electroporation with organotypic slice culture and time-lapse confocal imaging, which allows for a direct examination and dynamic analysis of radially migrating cortical neurons. Furthermore, detailed characterization of migrating neurons, such as migration speed, speed profiles, as well as radial orientation changes, is possible. The method can easily be adapted to perform functional analyses of genes of interest in radially migrating cortical neurons by loss and gain of function as well as rescue experiments. Time-lapse imaging of migrating neurons is a state-of-the-art technique that once established is a potent tool to study the development of the cerebral cortex in mouse models of neuronal migration disorders.

Time-lapse Confocal Imaging of Migrating Neurons in Organotypic Slice Culture of Embryonic Mouse Brain Using In Utero Electroporation

This protocol provides instructions for direct observation of radially migrating cortical neurons. In utero electroporation, organotypic slice culture, and time-lapse confocal imaging are combined to directly and dynamically study the effects of overexpression or downregulation of genes of interest in migrating neurons and to analyze their differentiation during development.

זמן לשגות Confocal הדמיה של נוירונים נודדים תרבות פרוסה Organotypic של המוח עכבר עובריים באמצעות<em&gt; באוטרו</em&gt; Electroporation

In utero electroporation is a rapid and powerful approach to study the process of radial migration in the cerebral cortex of developing mouse embryos. It ...

Simple Generation of a High Yield Culture of Induced Neurons from Human Adult Skin Fibroblasts

Induced neurons (iNs), the product of somatic cells directly converted to neurons, are a way to obtain patient-derived neurons from tissue that is easily accessible. Through this route, mature neurons can be obtained in a matter of a few weeks. Here, we describe a straightforward and rapid one-step protocol to obtain iNs from dermal fibroblasts obtained through biopsy samples from adult human donors. We explain each step of the process, including the maintenance of the dermal fibroblasts, the freezing procedure to build a stock of the cell line, seeding of the cells for reprogramming, as well as the culture conditions during the conversion process. In addition, we describe the preparation of glass coverslips for electrophysiological recordings, long-term coating conditions, and fluorescence activated cell sorting (FACS). We also illustrate examples of the results to be expected. The protocol described here is easy to perform and can be applied to human fibroblasts derived from human skin biopsies from patients with various different diagnoses and ages. This protocol generates a sufficient amount of iNs which can be used for a wide array of biomedical applications, including disease modeling, drug screening, and target validation.

Direct neuronal reprogramming generates neurons that maintain the age of the starting somatic cell. Here, we describe a single vector-based method to generate induced neurons from dermal fibroblasts obtained from adult human donors.

דור פשוטה של תרבות תשואה גבוהה של נוירונים המושרה מ Fibroblasts עור מבוגר

Induced neurons (iNs), the product of somatic cells directly converted to neurons, are a way to obtain patient-derived neurons from tissue that is easily ...

Isolation and Culture of Primary Neurons and Glia from Adult Rat Urinary Bladder

The lower urinary tract has two main functions, namely, periodic urine storage and micturition; these functions are mediated through central and peripheral neuroregulation. Although extensive research on the lower urinary tract nervous system has been conducted, most studies have focused on primary culture. This protocol introduces a method for the isolation and culture of bladder neurons and glia from Sprague&#8211;Dawley rats. In this method, the neurons and glia were incubated in a 37 &#176;C, 5% CO2 incubator for 5&#8211;7 days. As a result, they grew into mature shapes suitable for related subsequent immunofluorescence experiments. Cells were morphologically observed using an optical microscope. Neurons, synaptic vesicles, and glia were identified by &#946;-III-tubulin and MAP-2, Synapsin-1, and GFAP staining, respectively. Meanwhile, immunocytochemistry was performed on several neurotransmitter-related proteins, such as choline acetyltransferase, DYNLL2, and SLC17A9.

This protocol attempts to establish a repeatable protocol for primary neurons and glia isolation from rat bladder for further cellular experiments.

בידוד ותרבות של נוירונים ראשוניים גליה משלפוחית השתן של חולדה בוגרת

The lower urinary tract has two main functions, namely, periodic urine storage and micturition; these functions are mediated through central and ...

Culture of Neurospheres Derived from the Neurogenic Niches in Adult Prairie Voles

Neurospheres are primary cell aggregates that comprise neural stem cells and progenitor cells. These 3D structures are an excellent tool to determine the differentiation and proliferation potential of neural stem cells, as well as to generate cell lines than can be assayed over time. Also, neurospheres can create a niche (in vitro) that allows the modeling of the dynamic changing environment, such as varying growth factors, hormones, neurotransmitters, among others. Microtus ochrogaster (prairie vole) is a unique model for understanding the neurobiological basis of socio-sexual behaviors and social cognition. However, the cellular mechanisms involved in these behaviors are not well known. The protocol aims to obtain neural progenitor cells from the neurogenic niches of the adult prairie vole, which are cultured under non-adherent conditions, to generate neurospheres. The size and number of neurospheres depend on the region (subventricular zone or dentate gyrus) and sex of the prairie vole. This method is a remarkable tool to study sex-dependent differences in neurogenic niches in vitro and the neuroplasticity changes associated with social behaviors such as pair bonding and biparental care. Also, cognitive conditions that entail deficits in social interactions (autism spectrum disorders and schizophrenia) could be examined.

We established the conditions to culture neural progenitor cells from the subventricular zone and dentate gyrus of the adult brain of prairie voles, as a complementary in vitro study, to analyze the sex-dependent differences between neurogenic niches that could be part of functional plastic changes associated with social behaviors.

תרבות הנוירוספירות הנגזרות מהנישות הנוירוגניות בערבה בוגרת וול

Neurospheres are primary cell aggregates that comprise neural stem cells and progenitor cells. These 3D structures are an excellent tool to determine the ...

Single-Cell Electroporation across Different Organotypic Slice Culture of Mouse Hippocampal Excitatory and Class-Specific Inhibitory Neurons

Electroporation has established itself as a critical method for transferring specific genes into cells to understand their function. Here, we describe a single-cell electroporation technique that maximizes the efficiency (~80%) of in vitro gene transfection in excitatory and class-specific inhibitory neurons in mouse organotypic hippocampal slice culture. Using large glass electrodes, tetrodotoxin-containing artificial cerebrospinal fluid and mild electrical pulses, we delivered a gene of interest into cultured hippocampal CA1 pyramidal neurons and inhibitory interneurons. Moreover, electroporation could be carried out in cultured hippocampal slices up to 21 days in vitro with no reduction in transfection efficiency, allowing for the study of varying slice culture developmental stages. With interest growing in examining the molecular functions of genes across a diverse range of cell types, our method demonstrates a reliable and straightforward approach to in vitro gene transfection in mouse brain tissue that can be performed with existing electrophysiology equipment and techniques.

Presented here is a protocol for single-cell electroporation that can deliver genes in both excitatory and inhibitory neurons across a range of in vitro hippocampal slice culture ages. Our approach provides precise and efficient expression of genes in individual cells, which can be used to examine cell-autonomous and intercellular functions.

אלקטרופורציה חד-תאית על פני תרבות פרוסה אורגנוטיפית שונה של נוירונים מעכבים היפוקמפוס ומעמד ספציפיים

Electroporation has established itself as a critical method for transferring specific genes into cells to understand their function. Here, we describe a ...