EMMA Cryopreservation Workshop Novel concepts in mouse production and preservation

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EMMA Cryopreservation Workshop Novel concepts in mouse production and preservation Consejo Superior de Investigaciones Cientificas Madrid, Espagna May 7-8, 2012 K. C. Kent Lloyd, DVM, PhD University of California, Davis, USA

IMSR: 229,032 alleles* >16,000 genes (75% of genome) *Induced mutant strain resource, October 2011 Lines held only in private labs not included Also includes non-genomic alleles (Cre, Flp, lacz, etc) Academic, not-for-profit only (no commercial, for-profits)

Of these 229,032 alleles 22,034 mice and germplasm germline alleles 206,998 ES cells only 90% of alleles are NOT germline

Of these 22,034 germline alleles existing as mice and germplasm 3114 are live mice most also germplasm 18,920 (~86%) are only germplasm includes embryos and/or sperm Therefore, most germline alleles in repositories are in suspended animation, requiring recovery to live mice for use.

IKMC (INTERNATIONAL KNOCKOUT MOUSE CONSORTIUM) KOMP -C57BL6/N -lacz-tagged -K/O alleles: conditional null targeted trap deletion 17,000 genes Mutant ES cell resource 250-500 mutant mice/yr 8,500 genes (KOMP) 8,000 genes (EUCOMM) 500 genes (NorCOMM) + Vector resource

KOMP: Knockout Mouse Project KOMP2 KOMP1 2011-2021 ~US$275million 8500 mouse lines with phenotype 2006-2011 ~US$55million 8500 ES cell lines Nature Genetics 2004;36:921 In 2003, a meeting at the Banbury Center, Cold Spring Harbor developed a proposal for high throughput gene knockouts and phenotyping for every gene in the mouse genome KOMP

New frontiers in suspended animation Since 1972, embryo cryopreservation in liquid nitrogen has been the gold standard for preserving mutant mouse lines. Sperm cryopreservation receiving more attention Enhancements in techniques made to promote stability during storage, ensure viability upon recovery, reduce cost, increase speed, control quality, make reliable

Technological improvements that anticipate future needs Example: cumulative mutant mouse line orders (10 yrs) 300 Disruptive innovations 250 Traditional technology 200 150 100 50 0 1999 2000 2001 2002 2003 2004 2005 2006 2007 2008 2009 Live Mice Cryo Recovery Frozen Germplasm RATIONALE: 1-Live mice in most demand 2-Frozen formats are innovative, leading edge technology 3-Use of frozen formats mice reduces maintenance and distribution costs

Projects in progress -efficient derivation of ips cells from mutant lines -enhanced intracytoplasmic nuclear injection (ICNI) -targeting in mutant ips cells -restoring viability (e.g., motility) to dried sperm -mercury-free mechanical zona drilling (RosDrill c ) -molecular vectors as reliable (recoverable) genetic storage formats -warp-speed congenics

Procedure Preserve Maintain Recover Format Individual Lab self Type of User Transgenic facility intramural Repository extramural distribution Embryos Sperm ES cells Embryos Sperm ES cells Embryos Sperm ES cells Eg. Lab may want to preserve only (natural) embryos, not sperm Eg. Facility may want to preserve (mostly) embryos (IVF) and sperm (few slow, sure) Eg. Repository may want to preserve ESC & (mostly) sperm (many fast, cheap, versatile)

Technology enhancement: Protection against cryo induced oxidation damage of sperm B6.Cg-Mecp2 tm1.1jae /Mmcd: 24%* 41%* 30% 1% Other mutant strains: *Reproduction 2012 Mutant strain background C57BL/6J FVB/N CD1 Freezing Media No. mutant strains tested No. 2 cell embryos (%) CPM 20 604 (6%) CPM + MTG 13 627 (15%)* CPM 41 3990 (31%) CPM + MTG 30 5278 (52%)*

Technology replacement: Unconventional preservation of mouse sperm* In vitro development of embryos from ICSI using freeze-dried sperm: Genetic background B6D2F1/J C57BL/6J Treatment No. eggs survived No. 2 cell embryos (%) No. blastocysts (%) Fresh 75 70 (93%) 55 (73%) Freeze dried 77 68 (85%) 44 (57%) Fresh 59 51 (86%) 41 (69%) Freeze dried 52 47 (90%) 28 (54%) Genetic screening of 3 generations of mice from ICSI using freeze-dried sperm: Genetic No. MS alleles No. MS mutations Treatment P F1 F2 F3 background tested detected B6D2F1/J Natural mating 8 35 26 28 1424 0 Fresh ICSI 8 41 29 29 1584 0 Freeze dried ICSI 6 24 22 20 1056 0 C57BL/6J Natural mating 8 24 24 20 2176 0 Fresh ICSI 10 29 35 26 2880 0 Freeze dried ICSI 8 20 19 18 1824 0 *Zygote, 2009

Technology improvement: Simpler, faster, cheaper sperm preservation by evaporative drying* B6.129P2-APOE tm1unc : *Reproduction 2012 Fresh Sperm ICSI Group ED Sperm ICSI Group No. oocytes injected 380 364 No. oocytes survived ICSI 149 128 ICSI survival rate (%) 39.2% 35.2% No. 2 cell embryos obtained 137 114 Fertilization rate (%) 91.9% 89.1% No. pups born 52 20 Birth rate (%) 38.0% 17.5% Sex ratio (M/F) 25/27 12/8 Fresh Sperm ICSI Group ED Sperm ICSI Group No. natural mating pairs 5 6 No. of litters born 5 5 Litter rate 100% 83.3% No. pups born 30 28 Sex ratio (M/F) 13/17 17/11

Disruptive technology: Freezing & storage of somatic tissues/cells for rederivation* (Oct3/4, Sox2 and Klf4) ips cells from No. ips clones No. AP & SEA1 positive (%) Frozen tail (1 week) 38 31 (71%) Frozen fibroblasts (1 month) 15 11 (73%) *Trans Tech, 2011