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I'm sure this has come up before, but I can't locate it....Does anyone know if the aforementioned hybrids retain the pharyngeal plate??
"Forget pounds and ounces, I'm figuring displacement!"
If we accept that: MBG(+)FGSF(=)HBG(F1) And we surmise that: BG(>)HBG(F1) while GSF(<)HBG(F1) Would it hold true that: HBG(F1)(+)AM500(x)q.d.(=)1.5lbGRWT? PB answer: It depends.
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Chairman, Pond Boss Legacy award; Moderator; field correspondent Lunker
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Awesome question, and a post that I've been meaning to create for some time. Tony I don't think enough research has been performed to address the questions regarding inherited traits of BRES - RBG hybrids - but maybe we can work together to advance the research efforts.
Let me add a few for our experts they can hopefully address:
Does gender of parentage species play a factor on genes inherited?
After several generations of interbreeding, will subsequent generations adopt more BG or RES traits? [HBG following several generations of interbreeding assume GSF traits - what about BRES-RBG?]
Many men go fishing all of their lives without knowing that it is not fish they are after. ~ Henry David Thoreau
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Start with this from a 1972 study. Things have changed a lot since then but you can see the basics here. Back later with more.
LINKAGE RELATIONSHIPS OF SIX ENZYME LOCI IN INTERSPECIFIC SUNFISH HYBRIDS (GENUS LEPOMIS)* T. E. WHEAT2 AND G. S. WHITT3 Department of Zoology, University of Illinois, Urbana, Illinois 61801 and W. F. CHILDERS Section of Aquatic Biology, Illinois Natural History Survey, Urbana, Illinois 61801 Manuscript received December 19, 1972
Backcross hybrids produced from the bluegill, the red-ear sunfish, and their F, interspecific hybrid have been analyzed for the inheritance of six enzyme phenotypes.
From the analysis of the F, hybrids, we can conclude that all six loci are present and functional with both alleles at each locus being expressed to the same extent. Linkage analysis in backcross hybrids: Table 1 presents the frequencies of TABLE 1 Allele frequrncy: RB F, 8 X R 0 !tlnll-A >lD€l-R Est ro &PDII BPGDH Homozygotes 76 62 67 68 62 65 Heterozygotes 64 78 73 72 78 75 ISOZYMES IN SUNFISH HYBRIDS TABLE 2 Allele frequency: RB F, 8 x B 0 347 MDH-A MDH-B Est TO rrGPDH GPGDH Homozygotes 53 58 69 58 68 70 Heterozygotes 67 62 51 62 52 50 homozygotes and heterozygotes for all six markers among the progeny of 8 F, X 9 red-ear sunfish. Similar data for the mating 8 F, x P bluegill are given in Table 2. There is no significant deviation from the expected ratio of 1 homozygote to 1 heterozygote for each locus at the 99% significance level. However, it is possible that there is an increased frequency of the bluegill allele for aGPDH in both crosses reflected in excess homozygotes in the backcross to the bluegill, and excess heterozygotes in the mating with the red-ear sunfish. The excess of individuals receiving the bluegill allele from the Fl parent (146/114) is significant at less conservative confidence limits (x2 = 3.94; .01 < p < .05). These observations are consistent with the inheritance of the parentally derived genes as codominant alleles at nuclear loci. In addition, there are no apparent differences in viability between the two reciprocal backcrosses, confirming the suitability of this genetic system for linkage analysis. Tables 3 and 4 show the distributions of parental phenotypes and presumed recombinant classes for the fifteen pairs of markers in the matings of the F, hybrid with the red-ear sunfish and the bluegill, respectively. The x2 value is calculated for the deviation of the observed data from the 1:1:1:1 distribution TABLE 3 Linkage relationships: RB F, 8 X R 0 99p homA het A hom A het A Percent confi ence A B homB het B het B homB x2 recombination limit MDH-A MDH-B 33 35 43 29 .MO 51.4 10.9 MDH-A Est 32 29 44 35 2.20 56.4 10.8 MDH-A TO 39 35 37 29 .5ai 47.1 10.9 MDH-A 6PGDH 37 37 39 27 .616 47.1 10.9 MDH-A aGPDH 35 37 41 27 ,210 48.6 10.9 MDH-B Est 32 43 30 35 .629 46.4 10.9 MDH-B TO 31 41 31 37 .091 48.6 10.9 MDH-B 6PGDH 29 42 33 36 .005 49.3 10.9 MDH-B aGPDH 25 41 37 37 ,708 52.9 10.9 Est TO 29 34 38 39 1.44 55.0 10.8 Est 6PGDH 24 32 43 41 5.81 60.0 10.7 Est aGPDH 22 33 45 4.0 6.83 60.7 10.6 TO 6PGDH 32 39 36 33 .021 49.3 10.9 TO aGPDH 29 39 39 33 ,144 51.4 10.9 6PGDH* aGPDH 53 66 12 9 68.2 15.0 7.79 * These two loci show significant linkage. 348 T. E. WHEAT AND G. S. WHITT TABLE 4 Linkuge relationships: RB F, 8 X B Q A 99% homA hetA homA hetA Percent confidence B homB het B hetB homB x2 recombination limit MDH-A MDH-A MDH-A MDH-A MDH-A MDH-B MDH-B MDH-B MDH-B Est Est Est 6PGDH TO 6PGDH* MDH-B Est 6PGDH TO aGPDH Est 6PGDH TO (uGPDH GPGDH TO aGPDH TO aGPDH aGPDH 29 38 24 29 1.55 33 31 20 36 382 34 31 19 36 1.08 25 34 28 33 .051 29 28 24 39 .I47 36 29 22 33 ,959 33 25 25 37 .a95 24 28 34 34 2.17 28 22 30 40 3.22 45 26 24 25 3.16 30 23 39 28 1.53 45 28 24 23 4.84 27 19 43 31 6.41 31 25 27 37 ,474 56 38 I4 12 37.2 4.4.2 11.7 46.7 11.7 45.8 11.7 50.8 11.8 52.5 11.8 45.8 11.7 51.7 11.8 56.7 11.7 58.3 11.6 40.8 11.6 55.8 11.7 39.2 11.5 61.7 11.5 53.3 11.7 21.7 9.7 * These two loci show significant linkage. expected for unlinked loci. The frequency of recombination (MATHER19 51) and the confidence limit at the 99 % level are also presented. In both tables (3 and 4), there are no significant deviations (99% limit) from random assortment for the first fourteen pairs of markers; the frequencies of recombination are on the order of 50%. These data are not significantly different from the random assortment of codominant alleles at unlinked nuclear loci. However, loose linkage cannot be excluded. In contrast, for both backcrosses, GPGDH and (uGPDH show highly significant deviations from random assortment, and the calculation of the frequency of recombination confirms linkage between these two markers. The recombination values calculated for both backcrosses are not significantly different, so the true frequency of recombination is probably between 15% and 22%. Other possible deviations are found for Est-aGPDH in the backcross to the red-ear sunfish (x2 = 6.83; 0.01 < p < 0.05), and for GPGDH-TO in the backcross to the bluegill (x2 = 6.41; 0.01 < p < 0.05). In view of the large number of tests, it is probably better to consider only differences at the more conservative limit. In any case, these deviations could not reflect linkage since the observed frequency of recombination exceeds 0.5. DISCUSSION These data clearly demonstrate the utility of interspecific sunfish hybrids for genetic analysis. The viability of the interspecific hybrids and their progeny, as well as the large number of isozyme markers, is particularly advantageous. All six markers examined are inherited in a mendelian manner as codominant alleles at nuclear loci. There is no allelic repression detected in these interspecific ISOZYMES IN SUNFISH HYBRIDS 349 hybrids, although allelic inhibition has been observed for interspecific sunfish hybrids formed from more distantly related species (WHITTC, HOa nd CHILDERS 1972). No differential mortality was detected in either backcross population. Finally, no significant differences between the reciprocal crosses were detected. The slight excess of bluegill alleles for (rGPDH in both crosses probably reflects statistical variation due to the large number of tests being made. However, it may reflect differential mortality or some other distortion of the patterns of inheritance. Additional data would be necessary to clarify this point. The absence of close linkage between the MDH-A and MDH-B loci has been previously observed in the backcross between the RB F, hybrid and the red-ear sunfish (WHEATW, HITTa nd CHILDER1S9 72). This conclusion is confirmed by the present study. Since the two supernatant MDH loci (A and B) of teleosts are such closely homologous duplicate genes (BAILEY et al. 1970), the absence of close linkage may be of developmental or evolutionary significance. These data are consistent either with tandem duplication followed by some form of chromosomal rearrangement or with duplication during an ancient polyploidization event (OHNO 1970). The significance of the linkage of the loci encoding 6-phosphogluconate dehydrogenase and the liver form of a-glycerophosphate dehydrogenase for metabolic regulation is doubtful since the enzymes are in different metabolic pathways. These loci are unlinked in Drosophila (Fox, ABACHERLaIn d URSPRUNG19 71). Since recombination occurs with a frequency of 15 %-20% between these linked loci, recombination between the parental chromosomes in the F, hybrid is clearly demonstrated in this case. No data are available concerning the frequency of recombination between these loci in the parental species, so it cannot be determined whether the frequency of recombination is altered in the F, hybrid. Apart from its intrinsic genetic interest, the observation of linkage is of special significance to other studies of interspecific sunfish hybrids. The presence of linked enzyme loci should be very helpful in investigating the mechanisms of synchrony of gene function during development. In addition, the determination of the specificity of the mechanisms responsible for allelic repression in interspecific hybrids could be assessed with linked enzyme loci, The observations that recombination can occur between these linked loci in the F, hybrid, and that there is no substantial difference between the two backcross populations, clearly demonstrate the utility of this interspecific sunfish hybrid system for further genetic analyses.
Last edited by ewest; 06/10/13 03:34 PM.
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Keith - Still Lovin Livin https://youtu.be/o-R41Rfx0k0(a short video tribute to the PB members we met on our 5 week fishing adventure) Formerly: 2ac LMB,HSB,BG,HBG,RES
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Lunker
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Lunker
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Does anyone know if the aforementioned hybrids retain the pharyngeal plate?? Sparkie, I think if you examine the relationship between Linkage RB F, 8 X R 0 99p homA het A hom A het A Percent confidence A B homB het B het B homB x2 recombination limit, and TO aGPDH 29 39 39 33 ,144 51.4 10.9 6PGDH* aGPDH 53 66 12 9 68.2 15.0 7.79 with the assumption that at the 99% conidence limit, 29 38 24 29 1.55 33 31 20 36 382 34 31 19 36 1.08 25 34 28 33 .051 29 28 24 39 .I47 36 29 22 33 ,959 is not playing a limiting role, the answer is rather obvious: "Maybe". In the interest of applied, rather than pure, science, I would suggest the next set of videos posted by Gar King be of himself inserting his index finger into the pharyngeal space of several 1 pound RES vs BG hybrids. Examination of the condition of the retrieved digit should provide a definitive answer to this question, as well as bring forgiveness from Sunil for any future maceration of the english language.
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Eric, could you make a answer a little more complex. I hate such simple dribble. YS, thank you for my lottery numbers for the rest of the year. Maybe "Ruby Don't Take Your Loving To Town" would not have been so successful if Viagra had been available back then,"Maybe".
Two ponds, 13 and 15 acres on the Mattaponi River.
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Moderator Ambassador Field Correspondent  Lunker
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I nominate Yolk's post above for POTY.
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It all seems so simple when Yolk explains it. And to think I was about to demonstrate my ignorance for the entire world to see by asking ewest if his post was available in CliffsNotes....for those like me who don't make a living by speaking fish. Now THAT would've been embarrassing to admit.
Thanks for clearing that up and letting me save face Yolk!
"Forget pounds and ounces, I'm figuring displacement!"
If we accept that: MBG(+)FGSF(=)HBG(F1) And we surmise that: BG(>)HBG(F1) while GSF(<)HBG(F1) Would it hold true that: HBG(F1)(+)AM500(x)q.d.(=)1.5lbGRWT? PB answer: It depends.
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I nominate Yolk's post above for POTY. ...and I will probably embarrass myself by asking..... POTY???? That's not in the acronym list.
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Moderator Ambassador Field Correspondent  Lunker
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Moderator Ambassador Field Correspondent  Lunker
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I nominate Yolk's post above for POTY. ...and I will probably embarrass myself by asking..... POTY???? That's not in the acronym list. Made up on the fly. Post Of The Year.
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Moderator Hall of Fame 2014  Lunker
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If you want the study PM me an email address.  Did not have time to clean up the charts so they made sense. Point is this is very complex stuff with a lot of unknowns even at this point. I will put up some different info that is clearer.
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How about this: Can anyone post some photos of the pharyngeal plate/teeth of a RES? We have a number of these fish that occur naturally in our ponds, (I caught 4 nice specimens this weekend), and I will open some up and take a look.....provided I know what to look for. Ewest, thank you for your efforts. Much appreciated! 
"Forget pounds and ounces, I'm figuring displacement!"
If we accept that: MBG(+)FGSF(=)HBG(F1) And we surmise that: BG(>)HBG(F1) while GSF(<)HBG(F1) Would it hold true that: HBG(F1)(+)AM500(x)q.d.(=)1.5lbGRWT? PB answer: It depends.
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Moderator Hall of Fame 2014  Lunker
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Moderator Hall of Fame 2014  Lunker
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TEMPO OF HYBRID INVIABILITY IN CENTRARCHID FISHES
(TELEOSTEI: CENTRARCHIDAE)
DANIEL I. BOLNICK1,2 AND THOMAS J. NEAR3,4
Asymmetries in F1 Hybrid Viability
Centrarchid hybrid viability differs between reciprocal
crosses of the same pair of species (F1 asymmetry). Of 18
species pairs for which reciprocal crosses have been done
(and viability is nonzero), 17 had significantly different viabilities
depending on which species was the female (or male)
parent. The relative strength of this asymmetry increased linearly
with time (Fig. 4), because the absolute difference in
viabilities was fairly constant and represented an increasing
proportion of the overall viability as the latter measure declined.
Asymmetrical F1 viabilities may also result from deleterious
interactions between the maternally provided oocyte
cytoplasm and the hybrid’s nuclear genes. Centrarchid hybrids
show aberrant timing of allozyme gene expression during
early development, even when the parental species have
identical onset of gene expression (Phillip et al. 1983). These
results suggest that centrarchid species have diverged in their
gene regulation mechanisms even while expression location
and timing remained similar. In many cases, hybrids expressed
maternal alleles at the normal time, but paternally
derived alleles were delayed, premature, or failed to be expressed
at all (Phillip et al. 1983). Less viable hybrids in a
reciprocal cross are generally the ones with greater paternal
allele misexpression. Whitt et al. (1977) suggested that the
greater effect on paternal alleles is evidence for cytoplasmicnuclear
interactions, hypothesizing that maternally encoded
regulatory signals are misinterpreted by the paternal allele.
If one species’ gene expression is more sensitive to changes
in transcription factors, asymmetries will result.
One puzzling pattern
to emerge from our data lends some credence to a role for
cytonuclear interactions: using maximum body size as an
index (Page and Burr 1991), the larger species tends to be
the more successful maternal parent (Table 3). Of the 18
species pairs with reciprocal cross data and nonzero viability,
one pair had equal body size and nearly symmetrical crossing
success. Focusing on the remaining 17 species pairs (admittedly
not phylogenetically independent; Table 3), the larger
parent was more successful in 13 crosses and less successful
in four crosses (x12 5 4.765, P 5 0.029). We speculate that
there is greater disruption of paternal allele expression when
the paternal allele is from a smaller species, placed in an egg
with cytoplasmic factors encoded by a larger maternal species.
However, the cytoplasmic effect cannot be attributed to
differences in egg size, as egg size is not correlated with
body size (D. I. Bolnick, unpubl. data) and egg size differences
are not associated with inviability (Merriner 1971b).
We are working on expanding our dataset to include more
reciprocal crosses to test this pattern more rigorously
HAVING POSTED THIS ON CENTRAS NOTE THAT RES X BG SEEM TO BE THE EXCEPTION FOR SEVERAL REASONS INCLUDING NEAR SIMILAR SIZE OF THE TWO SPECIES AND DO CROSS WELL IN BOTH DIRECTIONS.
Last edited by ewest; 06/10/13 09:32 PM.
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How about this: Can anyone post some photos of the pharyngeal plate/teeth of a RES? We have a number of these fish that occur naturally in our ponds, (I caught 4 nice specimens this weekend), and I will open some up and take a look.....provided I know what to look for.
See this for info and pics http://intarch.ac.uk/journal/issue3/colburn/1intro.html
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Chairman, Pond Boss Legacy award; Moderator; field correspondent Lunker
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Tony please post pics of your BRES...or email them to me. Want to review and admire.
Many men go fishing all of their lives without knowing that it is not fish they are after. ~ Henry David Thoreau
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Moderator Lunker
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Well, now we understand why you have to hire a Lawyer to interpret the law.
It's not about the fish. It's about the pond. Take care of the pond and the fish will be fine. PB subscriber since before it was in color.
Without a sense of urgency, Nothing ever gets done.
Boy, if I say "sic em", you'd better look for something to bite. Sam Shelley Rancher and Farmer Muleshoe Texas 1892-1985 RIP Grandpa
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Lunker
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Lunker
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I wanted to revive this thread to see if any further info has been gathered, and get some ideas on what to look for or avoid if Bruce and I tackle a small (600 Sq Ft) breeding pond for male RES and female NBG.
Any input is appreciated.
Just a Pond Boss 'sponge'
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No additional information but sounds like an interesting project.
What are your goals and intentions for the offspring. I assume such a small pond the idea is to create hybrid offspring to stock somewhere else?
John
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Lunker
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Right now my plan is to create hybrid offspring and share them with TJ, Shorty, Bruce and any other local pond bossers to see how they respond. Just kids playing with toys essentially  Don't you come up this way in early September for Husker Harvest days? We may have to make arrangements to send a few home with you!!
Just a Pond Boss 'sponge'
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How many are you trying to produce? A small pond may be more than you need for the actual spawning part.
Aquaculture Cooperative Research / Extension Lincoln University of Missouri
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Lunker
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Lunker
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I have no limit on how many we want to produce. I'll throw a few in my .65 acre RES/SMB pond, give a few to Shorty, TJ and Bruce and then throw the rest in my 15 acre pond. I've just recently built a 600 sq ft pond and was going to put it to use growing out BG. Bruce suggested we grow out hybrids instead.
I sense you've got suggestion on how to do such in a tank as I've read a lot of your prior posts. I'd love to get some more detail on how to do such. I was hoping you'd chime in on this. Thanks for taking the time.
Just a Pond Boss 'sponge'
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You could get spawns off in a stock tank and transfer the prolarvae-laden nest(s) to ponds prepped for rearing. That would allow more control over numbers and 1 cohort so you can have 4" plus fish by the following fall that would require a lot less grading.
Aquaculture Cooperative Research / Extension Lincoln University of Missouri
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Lunker
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Lunker
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Tricks of the trade to get a spawn off in a stock tank?
Just a Pond Boss 'sponge'
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High school kids can do it so I would not say they are tricks. You could also do it in a larger aquarium. I can breed 2-lb sunfish in 75-gallon tanks without too much trouble.
Aquaculture Cooperative Research / Extension Lincoln University of Missouri
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Right now my plan is to create hybrid offspring and share them with TJ, Shorty, Bruce and any other local pond bossers to see how they respond. Just kids playing with toys essentially  Don't you come up this way in early September for Husker Harvest days? We may have to make arrangements to send a few home with you!! That would be neat. Yes I am planning on HHD. It is September 11-13th. Planning on looking you up too.
John
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Moderated by Bill Cody, Bruce Condello, catmandoo, Chris Steelman, Dave Davidson1, esshup, ewest, FireIsHot, Omaha, Sunil, teehjaeh57
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Koi
by PAfarmPondPGH69, October 22
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