Name: efficient generation of hipsc neural lineage specific knockin reporters using the crispr/cas9 and cas9 double nickase system
Uploaded: 2015-05-28T15:00:00
Description: Watch this Scientific Journal Video about Efficient Generation of hiPSC Neural Lineage Specific Knockin Reporters Using the CRISPR/Cas9 and Cas9 Double Nickase System at JoVE.com

This work was supported by the Department of Neurosurgery, Memorial Hermann Foundation Staman Ogilvie Fund, the Bentsen Stroke Center at the University of Texas Health Science Center at Houston, and Mission Connect TIRR Foundation.

1. Design and Vector Construction for Targeting Vectors
<ol>
	<li>Once the lineage specific marker is determined, locate the genomic sequence of the gene and design the homology arms accordingly. The length of 5&#8217; homology arm is ~1 kb and of 3&#8217; homology arm is ~1.5 kb (Figure 1).</li>
	<li>Tag the reporter cassette sequentially downstream of the genomic sequence right before the stop codon, by subcloning, so that the endogenous expression is not altered or disrupted. Link the reporter, or d...

<ol>
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Gene targeting is an essential tool in characterizing gene functions. However, the relatively low efficiency demands labor-intensive and time-consuming work. Recently development on genome editing tools such as the CRISPR (Clustered Regularly Interspaced Short Palindromic Repeats)/Cas (CRISPR-associated) system has greatly improved the targeting efficiency. This manuscript describes a protocol for generating lineage specific human induced pluripotent stem cell (hiPSC) reporter using CRISPR/Cas system assisted homologous recombination. Steps ...

CRISPR (אשכולות באופן קבוע Interspaced חזרות Palindromic קצרה) / קאש מערכת (הקשורים CRISPR), יחד עם כלי עריכת הגנום אחרים, יש מהפכה במניפולצית הגנום האנושית בשנים האחרונות 1-7. מרכיבים עיקריים במערכת / Cas9 CRISPR הם RNA מדריך יחיד (sgRNA) וCas9. Cas9 הוא הסוג השני endonuclease DNA מודרך RNA. יש לו שני תחומים nuclease, האמפ וRuvC, אשר אחראים על ביצוע הפסקות גדילי דנ&quot;א כפולים (DSBs) באזור גנומי ספציפי ליד מוטיב סמוך protospacer יש (PAM) 7-10 .An sgRNA פונקציה משולבת של זה של crRNA וtracrRNA, שתי מולקולות RNA הסתגלות חסינות שזוהו בחיידקים (כגון סטרפטוקוקוס pyogenes) וחיידקים קדומים להילחם נגד פלישת DNA של מקורות אקסוגניים 9-11. כאשר תוכנן כראוי ושיתוף הציג לתאי יונקים, sgRNA מכיר את רצף PAM, בסיס-זוגות עם הגדיל המשלים של ה- DNA היעד, ומדריכים וtransactivates Cas9 לדבוקבשני גדילי הדנ&quot;א באופן מיידי במעלה הזרם של 7 PAM. בהמשך לכך, בבימויו הומולוגי רקומבינציה (HDR, בנוכחותו של וקטור מיקוד) או בסוף שאינו הומולוגי שהצטרף (NHEJ) יתרחש לתקן DSBs. Transgenes כגון cDNAs, קלטות כתב, או שברים עמידים לאנטיביוטיקה יכול להיות משולב, וקווים מהונדסים או להתרפק עשו. למרות שהמערכה / Cas9 CRISPR היא יעילה ביותר ויחסית ספציפית, לא רצויה דווחו פעילויות מחוץ יעד 12-15. כדי למזער את האירועים מחוץ היעד, nickases Cas9 (Cas9n) יש גם מהונדס 9,10,14,16,17. Cas9n (D10A Cas9 או Cas9 H840A) הוא אנזים Cas9 עם מוטציות באחד משני תחומים nuclease, שמעורר רק ניק בגדיל אחד של DNA. כדי להשיג מחשוף בשני הגדילים, שתי sgRNAs נועד להדריך את זוג nickases, אשר חותך בנפרד בלוקוסים סמוכים של שני גדילי דנ&quot;א שונים. האסטרטגיה &quot;nicking הכפול&quot; דורשת מורעיצוב דואר מחמיר יותר מאשר פלטפורמת Cas9 הקונבנציונלית, ומציע גם יעילות גבוהה וסגוליים גבוהות לניסויי עריכת גן. כתב יד זה מתאר פרוטוקול להפקת כתב שושלת ספציפי בתאי גזע אנושיים pluripotent מושרה (hiPSC) באמצעות מערכת CRISPR / קאש סייעה רקומבינציה ההומולוגית. צעדים להשגת הרכיבים הדרושים להכנת קווי כתב שושלת עצבית באמצעות CRISPR / עריכת הגנום מערכת תיווך קאש מתוארות, עם דגש על הבנייה של וקטורי מיקוד וsgRNAs. פרוטוקול זה כבר חזר בהצלחה בשורות hiPSC מרובות כוללים אלה נגזרים מאנשים בריאים ומחולים במחלות של מערכת העצבים המרכזית. גנים ממוקדים במעבדה שלנו כוללים OLIG2, HB9 (MNX1), NEUROG2, SOX1, ALDH1L1 וSOD1. מיקוד יעילות מCRISPR מערכת / קאש בתיווך רקומבינציה ההומולוגית בhiPSCs נע בין 20-40%, אשר עולה בקנה אחד עם דיווחים קודמים 1,18,19. בהשוואה לtypicaיעילות l של 1-2% בניסויי גן המיקוד קונבנציונליים, יעילות המיקוד משופרת באופן משמעותי.

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efficient generation of hipsc neural lineage specific knockin reporters using the crispr/cas9 and cas9 double nickase system

מיקוד גן הוא גישה ביקורתית לאפיון פונקציות גן במחקר הביו-רפואי מודרני. עם זאת, היעילות של גן המיקוד בתאים אנושיים הייתה נמוכה, המונעת את הדור של שורות תאים אנושיות בקצב רצוי. בשנתיים האחרונות היינו עדים להתקדמות מהירה בשיפור היעילות של מניפולציה גנטית על ידי כלי עריכת הגנום כגון מערכת / קאש (הקשורים CRISPR) CRISPR (אשכולות באופן קבוע Interspaced חזרות Palindromic קצרה). כתב יד זה מתאר פרוטוקול להפקת כתבי שושלת ספציפיים בתאי גזע אנושיים pluripotent מושרה (hiPSC) באמצעות מערכת CRISPR / קאש סייעה רקומבינציה ההומולוגית. הליכים לקבלת רכיבים דרושים להכנת קווי כתב שושלת עצביים באמצעות CRISPR / מערכת קאש, תוך התמקדות בבנייה של וקטורי מיקוד וRNAs מדריך היחיד, מתוארים. פרוטוקול זה יכול להתארך עד הקמת פלטפורמה ותיקון מוטציה בhiPSCs.

Targeting vectors with all necessary components including homology arms, reporter cassette, positive and negative selection cassettes are constructed (Figure 1). Based on the endogenous genomic locus, multiple (2 to 3) sgRNAs (if using the Cas9 system) or sgRNA pairs (if using the Cas9n double nickase strategy) are designed and constructed into human-gRNA-expression vector MLM3636 or pX335-U6-Chimeric_BB-CBh-hSpCas9n (D10A) backbones (Figure 2). Before transfecting hiPSCs, the sgRNAs are...

Watch this Scientific Journal Video about Efficient Generation of hiPSC Neural Lineage Specific Knockin Reporters Using the CRISPR/Cas9 and Cas9 Double Nickase System at JoVE.com

Efficient Generation of hiPSC Neural Lineage Specific Knockin Reporters Using the CRISPR/Cas9 and Cas9 Double Nickase System (Video) | JoVE

Genome editing tools such as the CRISPR (Clustered Regularly Interspaced Short Palindromic Repeats)/Cas (CRISPR-associated) system have greatly improved gene targeting efficiency in human induced pluripotent stem cells (hiPSCs). This manuscript describes a protocol for generating lineage specific hiPSC reporter using CRISPR/Cas system assisted homologous recombination.

דור יעיל של כתבים במכות ספציפיים Lineage hiPSC עצבי באמצעות CRISPR / Cas9 ומערכת Nickase זוגי Cas9

Gene targeting is a critical approach for characterizing gene functions in modern biomedical research. However, the efficiency of gene targeting in human ...

Research

JoVE Journal

Developmental Biology

Efficient Generation of hiPSC Neural Lineage Specific Knockin Reporters Using the CRISPR/Cas9 and Cas9 Double Nickase System

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Lineage tracing experiments define the origin, fate and behavior of cells in a specific tissue or organism. This technique has been successfully applied ...

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