Team:UNIPV-Pavia/Calendar/July/settimana4

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Latest revision as of 16:54, 24 October 2010

JULY: WEEK 4

July, 19th

TECAN test showed that no RFP was produced from our parts, so all parts are potentially correct! For this reason we decided to sequence:

I14-1 (Forward)
I16-1 (Forward)
I17-1 (Forward)
I18-1 (Forward)
I19-1 (Forward)

We also sequenced:

I74C5-2 (Forward and Reverse)
I84C5-2 (Forward and Reverse)
I12-2 (Forward and Reverse)

These samples were prepared for sequencing (DNA was essicated) and sent to BMR genomics.

Trasformation of RING into:

BW25141 (pir+)
BW25142 (pir116)
BW23474 (pir116)
DH5alpha
MG1655

Cultures were plated on:

BW2514: Cm 34ug/ml
BW25142: Cm 34ug/ml
BW234741: Cm 34ug/ml
DH5alpha: Cm 12,5ug/ml
MG1655: Cm 12,5ug/ml

Inoculum of:

I3-1
I10-1
I12-2
I14-1
I17-1
<partinfo>BBa_J23110</partinfo>

in 5ml LB+Amp. Cultures were grown ON 37°C 220 rpm.

BW23473 arrived from Yale University on a paper disk. It was grown ON in 5ml L, at 37°C, 220 rpm.

^top

July, 20th

BW23474 transformed with <partinfo>BBa_J72007</partinfo>

DH5alpha transformed with <partinfo>BBa_J72007</partinfo>

Results for plates incubated ON, 37° C:

BW23474 (pir116): showed colonies
BW25141 (pir+): showed colonies
BW25142 (pir116): showed colonies
DH5alpha: didn't show colonies
MG1655: didn't show colonies (even if there were a very few colonies that we suppose integrated the resistance of RING to survive - or the plate antibiotic wasn't homogeneous)

BW23474 transformed with RING	BW25141 transformed with RING	BW25142 transformed with RING
DH5alpha transformed with RING	MG1655 transformed with RING

Single colonies were picked from plates and grown in LB+Cm at proper concentration. MG1655 colonies were let grow in LB+Cm to check if they integrated the Cm resistance of RING.

MiniPrep was performed on cultures incubated yesterday, with following yields:

Culture	Quantification
I10-1	117.8 ng/ul
I12-2	105,9 ng/ul
I3-1	166,0 ng/ul
I14-1	116,8 ng/ul
I17-1	189,5 ng/ul
<partinfo>BBa_J23110</partinfo>	169,9 ng/ul

We retrieved from our freezer the following MiniPreps, with quantifications:

Culture	Quantification
4C5	276 ng/ul
I16-1	68,4 ng/ul
I18-1	63,6 ng/ul
I19-1	58,8 ng/ul

Digestion of:

Culture	Kind	Final reaction volume (ul)	DNA (ul)	H20 (ul)	Enzyme 1	Enzyme 2	Buffer H
<partinfo>BBa_J23110</partinfo>	Vector	25	6	14,5	1 SpeI	1 PstI	2,5
I3-1	Vector	25	10,5	10	1 XbaI	1 PstI	2,5
4C5	Vector	25	3,6	16,9	1 EcoRI	1 PstI	2,5
I14-1	Insert	25	12,8	7,7	1 EcoRI	1 PstI	2,5
I16-1	Insert	25	12,5	8	1 EcoRI	1 PstI	2,5
I17-1	Insert	25	8	12,5	1 EcoRI	1 PstI	2,5
I18-1	Insert	25	13	7,5	1 EcoRI	1 PstI	2,5
I19-1	Insert	25	13	7,5	1 EcoRI	1 PstI	2,5
I12-2	Insert	25	14	6,5	1 EcoRI	1 PstI	2,5
I10-1	Insert	25	12,5	8	1 EcoRI	1 PstI	2,5

These parts were gel run/cut:

I3-1 (X-P)	5,9 ng/ul
<partinfo>BBa_J23110</partinfo> (S-P)	20,2 ng/ul
I14-1 (E-P)	13,0 ng/ul
I16-1 (E-P)	5,5 ng/ul
I17-1 (E-P)	11,9 ng/ul
I18-1 (E-P)	8,4 ng/ul
I19-1 (E-P)	4,4 ng/ul

4C5, I12-2 and I10-1 couldn't be extracted from gel, because bands were insignificant. For this reason we decided not to perform ligations involving I12-2 and I10-1 today. Luckily we retrieved from our freezer 4C5(E-P), so we could perform following ligations:

I15new=<partinfo>BBa_J23110</partinfo> (S-P) + I3-1 (X-P)
I14_4C5=I14(E-P)+4C5(E-P)
I16_4C5=I16(E-P)+4C5(E-P)
I17_4C5=I17(E-P)+4C5(E-P)
I18_4C5=I18(E-P)+4C5(E-P)
I19_4C5=I19(E-P)+4C5(E-P)

Ligations were incubated overnight at 16°C.

Glycerol stock for BW23473.

Our glycerol was contaminated, so we decided to prepare it again!

BW23474-RING was re-inoculated because it is still not grown.

We incoulated from glycerol stock (3ul in 2ml LB+Amp):

<partinfo>BBa_J23110</partinfo>
<partinfo>BBa_J23118</partinfo>
<partinfo>BBa_J23116</partinfo>
<partinfo>BBa_J23114</partinfo>
<partinfo>BBa_J23106</partinfo>
<partinfo>BBa_J23105</partinfo>
<partinfo>BBa_J23101</partinfo>
<partinfo>BBa_J23100</partinfo>
<partinfo>BBa_B0033</partinfo>

in order to perform a TECAN test tomorrow.

Inoculum of MC1061 in LB, PBHR68 in LB+Amp and <partinfo>BBa_T9002</partinfo> in LB+Amp to prepare competent cells tomorrow.

^top

July, 21st

This morning all cultures were grown:

BW25141-RING
BW25142-RING
BW23474-RING
BW23474-RING re.inoculated yesterday night (thrown away because unuseful)
MG1655-1
MG1655-2
MG1655-3
MG1655-4

For these 7 seven cultures glycerol stocks were prepared and stored at -80°C. Remaning 5 ml were used to perform MiniPrep.

After MiniPrep, purified DNA was quantified with NanoDrop.

Culture	Quantification
BW25141-RING	20,9 ng/ul
BW25142-RING	31,8 ng/ul
BW23474-RING	36,5 ng/ul
MG1655-1	3,5 ng/ul
MG1655-2	24 ng/ul
MG1655-3	10,6 ng/ul
MG1655-4	25,7 ng/ul

Digestion of:

Culture	Kind	Final reaction volume (ul)	DNA (ul)	H20 (ul)	Enzyme 1	Enzyme 2	Buffer B
MG1655-1	Screening	25	20	0,5	1 HindIII	1 HindIII	2,5
MG1655-2	Screening	25	10	10,5	1 HindIII	1 HindIII	2,5
MG1655-3	Screening	25	20	0,5	1 HindIII	1 HindIII	2,5
MG1655-4	Screening	25	10	10,5	1 HindIII	1 HindIII	2,5
BW25141-RING	Screening	25	10	10,5	1 HindIII	1 HindIII	2,5
BW25142-RING	Screening	25	8	12,5	1 HindIII	1 HindIII	2,5
BW23474-RING	Screening	25	8	12,5	1 HindIII	1 HindIII	2,5
<partinfo>BBa_J23116</partinfo> positive control	Screening	25	2	18,5	1 HindIII	1 HindIII	2,5

Today we also prepared competent cells for cultures inoculated yesterday:

<partinfo>BBa_T9002</partinfo> (already resistent to Ampicillin, grown in LB+Amp)
MC1061 (grown in LB with no antibiotic)
PBHR68 (already resistent to Ampicillin, grown in LB+Amp)

In the afternoon, we transformed our ligations: Trasformation of ligations in:

Ligation name	E. coli strain	Resistance
I15new=<partinfo>BBa_J23110</partinfo> (S-P) + I3-1 (X-P)	DH5alpha	Amp 100
I14_4C5=I14(E-P)+4C5(E-P)	DH5alpha	Amp 100+Cm 12,5
I16_4C5=I16(E-P)+4C5(E-P)	DH5alpha	Amp 100 + Cm 12,5
I17_4C5=I17(E-P)+4C5(E-P)	DH5alpha	Amp 100 + Cm 12,5
I18_4C5=I18(E-P)+4C5(E-P)	DH5alpha	Amp 100 + Cm 12,5
I19_4C5=I19(E-P)+4C5(E-P)	DH5alpha	Amp 100 + Cm 12,5

Plates were incubated overnight at 37°C.

^top

July, 22nd

Plates results were not nice: I15 new showed few colonies (about 20 colonies), I14_4C5 showed 2 colonies, I16_4C5 showed 3 colonies and I18_4C5 1 colony, while for other plates no colony was observed, probably due to the fact that our 4C5 (E-P) plasmid retrieved from freezer was too old and not usable anymore. For this reason, we decided to perform a colony PCR on available colonies of I14_4C5, I16_4C5 and I18-4C5, on 3 colonies of I15new and to repeat wrong ligations and the one including I10-1 and I12-2 (their vector had to be changed with pSB4C5). Colonies were saved in 1ml LB+suitable antibiotic/s. After gel results positive colonies will be glycerol stocked.

Colony PCR of colonies picked from plates

Colony PCR and gel run showed that I15-1, I15-2 and I15-3 have the right insert. Also for I14_4C5-1 and I14_4C5-2 the insert was visible. For these parts we decided to perform a NheI-PstI screening. I16-4C5-1 and I16_4C5-3 showed the insert, so they will be screened as before. No band was observed for I16_4C5-2 and I18_4C5-1 (This ligation will be repeated).

Glycerol stok was prepared for I14_4C5-1, I14_4C5-2, I16_4C5-1, I16_4C5-3, I15new-1, I15new-2 and I15new-3. Falcon tubes containing the remaining culture were re-filled with 5ml LB+antibiotic and tomorrow will be screened.

Other parts (I14 E-P, I16 E-P, I17 E-P, I18E-P, I19 E-P) were available in the freezer, so only 3 parts still had to be digested. Digestion of pSB4C5 (E-P), I12-2(E-P) and I10-1(E-P) was repeated as yesterday, digestions were gel run/cut and bands were visible, so this time gel extraction was performed with the following quantifications:

pSB4C5 (E-P): 23,0 ng/ul
I10-1 (E-P): 14,1 ng/ul
I12-2 (E-P): 21,9 ng/ul

Following ligations were performed:

I17_4C5=I17(E-P)+4C5(E-P)
I18_4C5=I18(E-P)+4C5(E-P)
I19_4C5=I19(E-P)+4C5(E-P)
I10-4C5=I10(E-P)+4C5(E-P)
I12-4C5=I12(E-P)+4C5(E-P)

In the afternoon, competent T9002 (on LB+Amp+Cm 12,5 LB agar plates) and MC1061 (on LB+Cm 12,5 agar plates) cells were transformed with a negative control (ENTERO 4C5) in pSB4C5, in order to evaluate transformation efficiency. Plates were incubated at 37°C overnight.

We also performed a TECAN test in order to evaluate the ranking of sternght of promoters we inoculaed yesterday. Results how that the ranking is the one reported here (from stronger to weaker):

<partinfo>BBa_J23100</partinfo>
<partinfo>BBa_J23101</partinfo>
<partinfo>BBa_J23110</partinfo>
<partinfo>BBa_J23118</partinfo>
<partinfo>BBa_J23106</partinfo>
<partinfo>BBa_J23105</partinfo>
<partinfo>BBa_J23116</partinfo>
<partinfo>BBa_J23114</partinfo>

Today we also prepared new plates, because we finished the one prepared, for our intensive lab activity... 50 plates LB+Amp+Cm 12,5.

We transformed pSB4C5 (4ng) in our home made competent cells:

T9002
MC1061
PBHR68

to evaluate transformation efficiency.

^top

July, 23rd

All plates incubated yesterday (T9002-4C5, MC1051-4C5 and PBHR68-4C5) showed colonies! We decided to incubate T9002 for furthrt time, because colonies were too small, before counting... Soon we will count colonies to evaluate efficiency of transformation for our home made competent cells!

Today we transformed our ligations:

Ligation name	E. coli strain	Resistance
I17_4C5= I17 (E-P) + pSB4C5 (E-P)	DH5alpha	Cm 12,5
I18_4C5= I18 (E-P) + pSB4C5 (E-P)	DH5alpha	Cm 12,5
I19_4C5= I19 (E-P) + pSB4C5 (E-P)	DH5alpha	Cm 12,5
I10_4C5= I0 (E-P) + pSB4C5 (E-P)	TOP10	Cm 12,5
I12_4C5= I12 (E-P) + pSB4C5 (E-P)	TOP10	Cm 12,5
Entero 4C5	PBHR68	Amp 100+Cm 12,5
RING	MC1061	Cm 12,5
No DNA (negative control)	MC1061	Cm 12,5

After MiniPrep, purified DNA was quantified with NanoDrop.

Culture	Quantification
I15-1	34,2 ng/ul
I15-2	57,1 ng/ul
I15-3	72 ng/ul
I14_4C5-1	14,7 ng/ul
I14_4C5-2	20,9 ng/ul
I16_4C5-1	16,3 ng/ul
I16_4C5-2	15,3 ng/ul

Digestion of:

Culture	Kind	Final reaction volume (ul)	DNA (ul)	H20 (ul)	Enzyme 1	Enzyme 2	Buffer B
I15-1	Screening	25	3	18,5	0,5 NheI	0,5 PstI	2,5
I15-2	Screening	25	3	18,5	0,5 NheI	0,5 PstI	2,5
I15-3	Screening	25	3	18,5	0,5 NheI	0,5 PstI	2,5
I14_4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I14_4C5-2	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I16_4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I16_4C5-2	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5

Digestions were incubated for 3h at 37°C, then gel run.

Screening for I15, I14-4C5 and I16_4C5

Gel showed that all parts were ok!!

We also received sequencing results:

I14-1	correct!
I16-1	correct!
I17-1	correct!
I18-1	correct!
I19-1	correct!
I12-2	correct!
I7_4C5-2	correct!
I8_4C5-2	correct!

Our plate with MC1061 transformed with RING showed few contamination, so we decided to repeat the transformation.

^top

July, 24th

We retransformed RING in MC1061 in order to see if contamination we noticed yesterday was due to tranformation or not. Plate was incubated overnight at 37°C and tomorrow we will evaluate efficiency.

For plates incubated yesterday, we picked 2 colonies for each plate:

I10_4C5-1
I10_4C5-2
I12_4C5-1
I12_4C5-2
I17_4C5-1
I17_4C5-2
I18_4C5-1
I18_4C5-2
I19_4C5-1
I19_4C5-2

Efficiency of transformation:

Culture	Colonies
BW25141	232 colonies
BW25142	137 colonies
BW23474	1436 colonies

^top

July, 25th

The plate containing RING in MC1061 showed 3 colonies! These colonies were screened and grown in LB+Cm 12,5. For colonies picked yesterday screening digestion was performed. MiniPrep was performed for:

I10_4C5-1
I10_4C5-1
I12_4C5-1
I12_4C5-1
I17_4C5-1
I17_4C5-1
I18_4C5-1
I18_4C5-1
I19_4C5-1
I19_4C5-1

Digestion of:

Culture	Kind	Final reaction volume (ul)	DNA (ul)	H20 (ul)	Enzyme 1	Enzyme 2	Buffer Tango
I10-4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I10-4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I12-4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I12_4C5-2	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I17_4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I17_4C5-2	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I18_4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I18_4C5-2	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I19_4C5-1	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5
I19_4C5-2	Screening	25	10	11,5	0,5 NheI	0,5 PstI	2,5

Screening for I10_4C5, I12_4C5, I17_4C5, I18_4C5 and I19_4C5

From gel it is possible to see that all of them are positive!! :)

^top

@@ Line 32: / Line 32: @@
 <br>
 <html><p align="center"><font size="4"><b>JULY: WEEK 4</b></font></p></html><hr><br>
+<html><a name="indice"/></html>
 ==July, 19th==
@@ Line 74: / Line 75: @@
 BW23473 arrived from Yale University on a paper disk. It was grown ON  in 5ml L, at 37°C, 220 rpm.
+<div align="right"><small>[[#indice|^top]]</small></div>
 ==July, 20th==
@@ Line 210: / Line 213: @@
 Inoculum of MC1061 in LB, PBHR68 in LB+Amp and <partinfo>BBa_T9002</partinfo> in LB+Amp to prepare competent cells tomorrow.
-==July, 21st==
+<div align="right"><small>[[#indice|^top]]</small></div>
-<font size=4>[[Team:UNIPV-Pavia/Material Methods/Measurements/Tecan/test5|Tecan Test]]</font>
+==July, 21st==
 This morning all cultures were grown:
 *BW25141-RING
@@ Line 330: / Line 333: @@
 </table>
-Plates were incubated overnight at 37°C 220 rpm.
+Plates were incubated overnight at 37°C.
+<div align="right"><small>[[#indice|^top]]</small></div>
 ==July, 22nd==
-plates results were not nice: I15 new showed few colonies (about 20 colonies), I14_4C5 showed 2 colonies, I16_4C5 showed 3 colonies and I18_4C5 1 colony, while for other plates no colony was observed, probably due to the fact that our 4C5 (E-P) plasmid retrieved from freezer was too old and not usable anymore. For this reason, we decided to perform a colony PCR on available colonies of I14_4C5, I16_4C5 and I18-4C5, on 3 colonies of I15new and to repeat wrong ligations and the one including I10-1 and I12-2 (their vector had to be changed with pSB4C5).
+Plates results were not nice: I15 new showed few colonies (about 20 colonies), I14_4C5 showed 2 colonies, I16_4C5 showed 3 colonies and I18_4C5 1 colony, while for other plates no colony was observed, probably due to the fact that our 4C5 (E-P) plasmid retrieved from freezer was too old and not usable anymore. For this reason, we decided to perform a colony PCR on available colonies of I14_4C5, I16_4C5 and I18-4C5, on 3 colonies of I15new and to repeat wrong ligations and the one including I10-1 and I12-2 (their vector had to be changed with pSB4C5).
 Colonies were saved in 1ml LB+suitable antibiotic/s. After gel results positive colonies will be glycerol stocked.
-[[Image:UNIPV10_colony_pcr_I15new_I14-18.jpg|thumb|200px|center|Colony PCR of colonies peaked from plates]]
+[[Image:UNIPV10_colony_pcr_I15new_I14-18.jpg|thumb|200px|center|Colony PCR of colonies picked from plates]]
 Colony PCR and gel run showed that I15-1, I15-2 and I15-3 have the right insert. Also for I14_4C5-1 and I14_4C5-2 the insert was visible. For these parts we decided to perform a NheI-PstI screening. I16-4C5-1 and I16_4C5-3 showed the insert, so they will be screened as before. No band was observed for I16_4C5-2 and I18_4C5-1 (This ligation will be repeated).
@@ Line 380: / Line 385: @@
 *PBHR68
 to evaluate transformation efficiency.
+<div align="right"><small>[[#indice|^top]]</small></div>
 ==July, 23rd==
@@ Line 399: / Line 406: @@
 </td>
 <td>Cm 12,5</td>
-</tr><tr><td>
+</tr>
+<tr>
+<td>
 *I18_4C5= I18 (E-P) + pSB4C5 (E-P)
 </td>
@@ Line 406: / Line 415: @@
 </td>
 <td>Cm 12,5</td>
-</tr><tr><td>
+</tr>
+<tr>
+<td>
 *I19_4C5= I19 (E-P) + pSB4C5 (E-P)</td>
 <td>
@@ Line 412: / Line 423: @@
 </td>
 <td>Cm 12,5</td>
-</tr><tr><td>
+</tr>
+<tr>
+<td>
 *I10_4C5= I0 (E-P) + pSB4C5 (E-P)</td>
 <td>
@@ Line 418: / Line 431: @@
 </td>
 <td>Cm 12,5</td>
-</tr><tr><td>
+</tr>
+<tr>
+<td>
 *I12_4C5= I12 (E-P) + pSB4C5 (E-P)</td>
 <td>
@@ Line 424: / Line 439: @@
 </td>
 <td>Cm 12,5</td>
-</tr><tr><td>
+</tr>
+<tr>
+<td>
 *Entero 4C5</td>
 <td>
@@ Line 431: / Line 448: @@
 <td>Amp 100+Cm 12,5</td>
 </tr>
-</tr><tr><td>
+<tr>
+<td>
 *RING</td>
 <td>
@@ Line 438: / Line 456: @@
 <td>Cm 12,5</td>
 </tr>
-</tr><tr><td>
+<tr><td>
 *No DNA (negative control)</td>
 <td>
@@ Line 526: / Line 544: @@
 Our plate with MC1061 transformed with RING showed few contamination, so we decided to repeat the transformation.
+<div align="right"><small>[[#indice|^top]]</small></div>
 ==July, 24th==
@@ Line 554: / Line 574: @@
 |BW23474 || 1436 colonies
 |}
+<div align="right"><small>[[#indice|^top]]</small></div>
 ==July, 25th==
+The plate containing RING in MC1061 showed 3 colonies! These colonies were screened and grown in LB+Cm 12,5. For colonies picked yesterday  screening digestion was performed.
+MiniPrep was performed for:
+*I10_4C5-1
+*I10_4C5-1
+*I12_4C5-1
+*I12_4C5-1
+*I17_4C5-1
+*I17_4C5-1
+*I18_4C5-1
+*I18_4C5-1
+*I19_4C5-1
+*I19_4C5-1
+Digestion of:
+{| border='1'
+|  ''Culture''    ||   ''Kind''   ||  ''Final reaction volume (ul) '' ||  ''DNA (ul)''  ||  ''H20 (ul)''  ||   ''Enzyme 1''  ||  ''Enzyme 2'' ||   ''Buffer Tango''
+|-
+|  I10-4C5-1 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I10-4C5-1 ||  Screening || 25 ||  10  ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+| I12-4C5-1||  Screening || 25 ||  10  ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I12_4C5-2 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I17_4C5-1 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I17_4C5-2 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I18_4C5-1 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I18_4C5-2 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I19_4C5-1 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|-
+|  I19_4C5-2 ||  Screening || 25 ||  10   ||   11,5   ||      0,5 NheI  || 0,5 PstI   || 2,5
+|}
+[[Image:UNIPV10_II10_12_17_18_19_4C5_screening.jpg|thumb|200px|center|Screening for I10_4C5, I12_4C5, I17_4C5, I18_4C5 and I19_4C5]]
+From gel it is possible to see that all of them are positive!! :)
+<div align="right"><small>[[#indice|^top]]</small></div>
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